US20230420137A1

Cancer Score for Assessment and Response Prediction from Biological Fluids

Publication

Country:US
Doc Number:20230420137
Kind:A1
Date:2023-12-28

Application

Country:US
Doc Number:18465868
Date:2023-09-12

Classifications

IPC Classifications

G16H50/20G16H20/40G16H70/60G16H10/40G16H10/60G16H50/30G16H50/70G16H20/10G16B20/20G16B20/10

CPC Classifications

G16H50/20G16H20/40G16H70/60G16H10/40G16H10/60G16B25/10G16H50/70G16H20/10G16B20/20G16B20/10G16H50/30

Applicants

Nantomics, LLC

Inventors

Shahrooz Rabizadeh, Patrick Soon-Shiong

Abstract

Methods for analyzing omics data and using the omics data to determine prognosis of a cancer, to predict an outcome of a treatment, and/or to determine an effectiveness of a treatment are presented. In preferred methods, blood from a patient having a cancer or suspected to have a cancer is obtained and blood omics data for a plurality of cancer-related, inflammation-related, or DNA repair-related genes are obtained. A cancer score can be calculated based on the omics data, which then can be used to provide a cancer prognosis, a therapeutic recommendation, an effectiveness of a treatment.

Description

[0001]This application is a divisional application of allowed US application having Ser. No. 16/754,088, which was filed Apr. 6, 2020, and which is a 371 application of PCT/US2018/055481, which was filed Oct. 11, 2018, and which claims priority to US provisional application having the Ser. No. 62/571,414, filed Oct. 12, 2017, all of which are incorporated by reference in their entirety herein.

FIELD OF THE INVENTION

[0002]The field of the invention is profiling of omics data as they relate to cancer, especially as it relates to the generation of indicators for cancer prognosis, prediction of treatment outcomes, and/or effectiveness of cancer treatments.

BACKGROUND OF THE INVENTION

[0003]The background description includes information that may be useful in understanding the present invention. It is not an admission that any of the information provided herein is prior art or relevant to the presently claimed invention, or that any publication specifically or implicitly referenced is prior art.

[0004]All publications and patent applications herein are incorporated by reference to the same extent as if each individual publication or patent application were specifically and individually indicated to be incorporated by reference. Where a definition or use of a term in an incorporated reference is inconsistent or contrary to the definition of that term provided herein, the definition of that term provided herein applies and the definition of that term in the reference does not apply.

[0005]Cancer is a multifactorial disease where many diverse genetic and environmental factors interplay and contribute to the development and outcome of the disease. In addition, genetic and environmental factors often affect the patient's prognosis in various degrees such that individual patients may show different responses to the same therapeutic and/or prophylactic treatment. Such complexity and diversity render traditional prediction of prognosis, identification of optimal treatments, and prediction of likelihood of success of the treatments based on a single or few factors (e.g., serum level of inflammation-related proteins, etc.), often unreliable. Further, many traditional methods of examining such factors are invasive as they require tumor biopsy samples for histology of tumor cells and tissues.

[0006]More recently, DNA or RNA populations present in the peripheral blood have drawn attention for analyzing genetic abnormalities associated with the cancer status. For example, U.S. Pat. No. 9,422,592 discloses the measurement of cell free RNA (cfRNA) of formulpeptide receptor gene (FPR1) and its association with the patient's risk for having lung cancer or non-small cell lung cancer (NSCLC). Yet, such studies are limited to a few numbers of genes, which are typically weighed equally in determining the cancer status. As multiple factors affect to various degrees prognosis of most cancers, oversimplification may cause inaccurate prognosis and/or prediction of treatment outcome.

[0007]Thus, even though some examples of using cell free nucleic acid in determining cancer status are known, differentially weighed, multi-factor approaches in determining cancer status using cell free nucleic acid are largely unexplored. Thus, there remains a need for improved methods of analyzing omics data of cell free nucleic acids in determining status, prognosis of a cancer as well as likelihood of treatment outcome or effectiveness of the treatment.

SUMMARY OF THE INVENTION

[0008]The inventive subject matter is directed to methods of using various omics data of cell free nucleic acids to calculate a composite cancer score that can be used to determine the status, prognosis of a cancer as well as likelihood of treatment outcome and/or effectiveness of current treatments. Thus, one aspect of the subject matter includes a method of analyzing omics data. In this method, blood is obtained from a patient having or suspected to have a cancer. From the blood, omics data for a plurality of cancer-related genes are obtained. Most preferably, the omics data include at least one of DNA sequence data, RNA sequence data, and RNA expression level data. From the omics data, a composite score is calculated which can then be associated with at least one of a health status, an omics error status, a cancer prognosis, a therapeutic recommendation, and an effectiveness of a treatment.

[0009]In some embodiments, the DNA sequence data v selected from the group consisting of mutation data, copy number data duplication, loss of heterozygosity data, and epigenetic status. Optionally, the DNA sequence data is obtained from circulating free DNA. In other embodiments, the RNA sequence data is selected from the group consisting of mRNA sequence data and splice variant data, and/or the RNA expression level data is selected from the group consisting of a quantity of RNA transcript and a quantity of a small noncoding RNA. Optionally, the RNA sequence data is obtained from the group consisting of circulating tumor RNA and circulating free RNA.

[0010]Typically, the plurality of cancer-related genes comprises at least one of a cancer-related gene, a cancer-specific gene, a DNA-repair gene, a neoepitope, and a gene not associated with a disease. Preferably, the neoepitope is tumor-specific and patient-specific. In some embodiments, the plurality of cancer-related genes includes a cancer-specific gene, and the score is calculated based on a presence or an absence of a mutation in the cancer-specific gene. In such embodiments, it is preferred that the presence of the mutation in the cancer-specific gene weighs more than the presence of the mutation in the cancer-related genes other than the cancer-specific gene. In other embodiments, the score is calculated based on a type of a splice variant of the cancer gene or a ratio between or among a plurality of splice variants of the cancer gene.

[0011]In some embodiments, the method further comprises a step of comparing the score with a threshold value to thereby determine the therapeutic recommendation. In such embodiments, it is preferred that the therapeutic recommendation is a prophylactic treatment if the score is below the threshold value. Alternatively and/or additionally, the method further comprises a step of comparing the omics error status with a threshold value to thereby determine a risk score.

[0012]In another aspect of the inventive subject matter, the inventors contemplate a method of determining prognosis of a cancer of a patient. In this method, blood is obtained from a patient having or suspected to have a cancer. From the blood, omics data for a plurality of cancer genes are obtained. Preferably, the omics data include at least one of DNA sequence data, RNA sequence data, and RNA expression level data. From the omics data, a cancer prognosis score is calculated, and the prognosis of the cancer is provided based on the cancer prognosis score. IN some embodiments, the prognosis comprises a progress of metastasis.

[0013]In some embodiments, the DNA sequence data v selected from the group consisting of mutation data, copy number data duplication, loss of heterozygosity data, and epigenetic status. Optionally, the DNA sequence data is obtained from circulating free DNA. In other embodiments, the RNA sequence data is selected from the group consisting of mRNA sequence data and splice variant data, and/or the RNA expression level data is selected from the group consisting of a quantity of RNA transcript and a quantity of a small noncoding RNA. Optionally, the RNA sequence data is obtained from the group consisting of circulating tumor RNA and circulating free RNA.

[0014]Typically, the plurality of cancer-related genes comprises at least one of a cancer-related gene, a cancer-specific gene, a DNA-repair gene, a neoepitope, and a gene not associated with a disease. Preferably, the neoepitope is tumor-specific and patient-specific. In some embodiments, the plurality of cancer-related genes includes a cancer-specific gene, and the score is calculated based on a presence or an absence of a mutation in the cancer-specific gene. In other embodiments, the score is calculated based on a type of a splice variant of the cancer gene or a ratio among or between a plurality of splice variants of the cancer gene.

[0015]In some embodiments, the omics data is a plurality of sets of omics data obtained at a different time points during a time period, and the prognosis is provided based on a plurality of scores from the plurality of sets of omics data. In such embodiments, it is preferred that the prognosis is represented by a change of a plurality of scores during the time period, wherein the change is over a predetermined threshold value.

[0016]Still another aspect of inventive subject matter is directed towards a method of predicting an outcome of a treatment for a cancer patient. In this method, blood is obtained from a patient having a cancer. From the blood, omics data for a plurality of cancer genes are obtained. Preferably, the omics data include at least one of DNA sequence data, RNA sequence data, and RNA expression level data. From the omics data, a cancer gene score is calculated, and a predicted outcome of the treatment is provided based on the cancer prognosis score. Preferably, the predicted outcome is determined by comparing the cancer gene score with a predetermined threshold value.

[0017]In some embodiments, the treatment is a drug, and at least one of the plurality of cancer gene is a predicted target of the drug. In other embodiments, the treatment is an immune therapy, and at least one of the plurality of cancer gene is a receptor of an immune cell or a ligand of the receptor. In still other embodiments, the treatment is a surgery or a radiation therapy, and at least one of the plurality of cancer gene is a neoepitope that is tumor-specific and patient-specific.

[0018]In some embodiments, the DNA sequence data v selected from the group consisting of mutation data, copy number data duplication, loss of heterozygosity data, and epigenetic status. Optionally, the DNA sequence data is obtained from circulating free DNA. In other embodiments, the RNA sequence data is selected from the group consisting of mRNA sequence data and splice variant data, and/or the RNA expression level data is selected from the group consisting of a quantity of RNA transcript and a quantity of a small noncoding RNA. Optionally, the RNA sequence data is obtained from the group consisting of circulating tumor RNA and circulating free RNA.

[0019]Typically, the plurality of cancer-related genes comprises at least one of a cancer-related gene, a cancer-specific gene, a DNA-repair gene, a neoepitope, and a gene not associated with a disease. Preferably, the neoepitope is tumor-specific and patient-specific. In some embodiments, the plurality of cancer-related genes includes a cancer-specific gene, and the score is calculated based on a presence or an absence of a mutation in the cancer-specific gene. In other embodiments, the score is calculated based on a type of a splice variant of the cancer gene or a ratio between a plurality of splice variants of the cancer gene.

[0020]In still another aspect of the inventive subject matter, the inventors contemplate a method of evaluating an effectiveness of a treatment for a cancer patient. In this method, blood is obtained from a patient having a cancer. From the blood, omics data for a plurality of cancer genes are obtained before and after the treatment. Preferably, the omics data include at least one of DNA sequence data, RNA sequence data, and RNA expression level data. From the omics data, at least two cancer gene scores corresponding to the omics data before and after the treatment, respectively, are generated, and the effectiveness of the treatment is provided based on the comparison of the at least two cancer gene scores. In some embodiments, the effectiveness of the treatment can be determined by a difference between the cancer gene score before and after the treatment. In such embodiments, it is preferred that the treatment is determined effective when the difference is higher than a predetermined threshold value.

[0021]In some embodiments, the treatment is a drug, and at least one of the plurality of cancer gene is a predicted target of the drug. In other embodiments, the treatment is an immune therapy, and at least one of the plurality of cancer gene is a receptor of an immune cell or a ligand of the receptor. In still other embodiments, the treatment is a surgery or a radiation therapy, and at least one of the plurality of cancer gene is a neoepitope that is tumor-specific and patient-specific.

[0022]In some embodiments, the DNA sequence data v selected from the group consisting of mutation data, copy number data duplication, loss of heterozygosity data, and epigenetic status. Optionally, the DNA sequence data is obtained from circulating free DNA. In other embodiments, the RNA sequence data is selected from the group consisting of mRNA sequence data and splice variant data, and/or the RNA expression level data is selected from the group consisting of a quantity of RNA transcript and a quantity of a small noncoding RNA. Optionally, the RNA sequence data is obtained from the group consisting of circulating tumor RNA and circulating free RNA.

[0023]Typically, the plurality of cancer-related genes comprises at least one of a cancer-related gene, a cancer-specific gene, a DNA-repair gene, a neoepitope, and a gene not associated with a disease. Preferably, the neoepitope is tumor-specific and patient-specific. In some embodiments, the plurality of cancer-related genes includes a cancer-specific gene, and the score is calculated based on a presence or an absence of a mutation in the cancer-specific gene. In other embodiments, the score is calculated based on a type of a splice variant of the cancer gene or a ratio between a plurality of splice variants of the cancer gene.

[0024]Various objects, features, aspects and advantages of the inventive subject matter will become more apparent from the following detailed description of preferred embodiments.

DETAILED DESCRIPTION

[0025]The inventors discovered that the status and/or prognosis of a cancer can be more reliably determined in a less invasive and quick manner using a compound score that is generated based on multiple factors associated with the cancer. The inventors also discovered that the compound score can be used to reliably predict a likelihood of outcome of a cancer treatment, and further, effectiveness of a particular cancer treatment. Viewed from a different perspective, the inventors discovered that a compound score can be generated from the patient's omics data obtained from nucleic acids in the patient's blood. Typically the omics data include omics data of various cancer-related genes, which can be differentially weighed based on the type and timing of the sampling. The compound score can be a reliable indicator to determine cancer status and/or prognosis of a cancer, a likelihood of outcome of a cancer treatment. Further, the compound scores generated based on omics data obtained before and after a cancer treatment can be compared to determine the effectiveness of a cancer treatment.

[0026]As used herein, the term “tumor” refers to, and is interchangeably used with one or more cancer cells, cancer tissues, malignant tumor cells, or malignant tumor tissue, that can be placed or found in one or more anatomical locations in a human body.

[0027]It should be noted that the term “patient” as used herein includes both individuals that are diagnosed with a condition (e.g., cancer) as well as individuals undergoing examination and/or testing for the purpose of detecting or identifying a condition. Thus, a patient having a tumor refers to both individuals that are diagnosed with a cancer as well as individuals that are suspected to have a cancer.

[0028]As used herein, the term “provide” or “providing” refers to and includes any acts of manufacturing, generating, placing, enabling to use, transferring, or making ready to use.

Cell-Free DNA/RNA

[0029]The inventors contemplate that tumor cells and/or some immune cells interacting or surrounding the tumor cells release cell free DNA/RNA to the patient's bodily fluid, and thus may increase the quantity of the specific cell free DNA/RNA in the patient's bodily fluid as compared to a healthy individual. As used herein, the patient's bodily fluid includes, but is not limited to, blood, serum, plasma, mucus, cerebrospinal fluid, ascites fluid, saliva, and urine of the patient. Alternatively, it should be noted that various other bodily fluids are also deemed appropriate so long as cell free DNA/RNA is present in such fluids. The patient's bodily fluid may be fresh or preserved/frozen. Appropriate fluids include saliva, ascites fluid, spinal fluid, urine, etc., which may be fresh or preserved/frozen.

[0030]The cell free RNA may include any types of DNA/RNA that are circulating in the bodily fluid of a person without being enclosed in a cell body or a nucleus. Most typically, the source of the cell free DNA/RNA is the tumor cells. However, it is also contemplated that the source of the cell free DNA/RNA is an immune cell (e.g., NK cells, T cells, macrophages, etc.). Thus, the cell free DNA/RNA can be circulating tumor DNA/RNA (ctDNA/RNA) and/or circulating free DNA/RNA (cf DNA/RNA, circulating nucleic acids that do not derive from a tumor). While not wishing to be bound by a particular theory, it is contemplated that release of cell free DNA/RNA originating from a tumor cell can be increased when the tumor cell interacts with an immune cell or when the tumor cells undergo cell death (e.g., necrosis, apoptosis, autophagy, etc.). Thus, in some embodiments, the cell free DNA/RNA may be enclosed in a vesicular structure (e.g., via exosomal release of cytoplasmic substances) so that it can be protected from nuclease (e.g., RNAase) activity in some type of bodily fluid. Yet, it is also contemplated that in other aspects, the cell free DNA/RNA is a naked DNA/RNA without being enclosed in any membranous structure, but may be in a stable form by itself or be stabilized via interaction with one or more non-nucleotide molecules (e.g., any RNA binding proteins, etc.).

[0031]It is contemplated that the cell free DNA/RNA can be any type of DNA/RNA which can be released from either cancer cells or immune cell. Thus, the cell free DNA may include any whole or fragmented genomic DNA, or mitochondrial DNA, and the cell free RNA may include mRNA, tRNA, microRNA, small interfering RNA, long non-coding RNA (lncRNA). Most typically, the cell free DNA is a fragmented DNA typically with a length of at least 50 base pair (bp), 100 base pair (bp), 200 bp, 500 bp, or 1 kbp. Also, it is contemplated that the cell free RNA is a full length or a fragment of mRNA (e.g., at least 70% of full-length, at least 50% of full length, at least 30% of full length, etc.). While cell free DNA/RNA may include any type of DNA/RNA encoding any cellular, extracellular proteins or non-protein elements, it is preferred that at least some of cell free DNA/RNA encodes one or more cancer-related proteins, or inflammation-related proteins. For example, the cell free DNA/mRNA may be full-length or fragments of (or derived from the) cancer related genes including, but not limited to ABL1, ABL2, ACTB, ACVR1B, AKT1, AKT2, AKT3, ALK, AMER11, APC, AR, ARAF, ARFRP1, ARID1A, ARID1B, ASXL1, ATF1, ATM, ATR, ATRX, AURKA, AURKB, AXIN1, AXL, BAP1, BARD1, BCL2, BCL2L1, BCL2L2, BCL6, BCOR, BCORL1, BLM, BMPR1A, BRAF, BRCA1, BRCA2, BRD4, BRIP1, BTG1, BTK, EMSY, CARD11, CBFB, CBL, CCND1, CCND2, CCND3, CCNE1, CD274, CD79A, CD79B, CDC73, CDH1, CDK12, CDK4, CDK6, CDK8, CDKN1A, CDKN1B, CDKN2A, CDKN2B, CDKN2C, CEA, CEBPA, CHD2, CHD4, CHEK1, CHEK2, CIC, CREBBP, CRKL, CRLF2, CSF1R, CTCF, CTLA4, CTNNA1, CTNNB1, CUL3, CYLD, DAXX, DDR2, DEPTOR, DICER1, DNMT3A, DOT1L, EGFR, EP300, EPCAM, EPHA3, EPHA5, EPHA7, EPHB1, ERBB2, ERBB3, ERBB4, EREG, ERG, ERRFIL ESR1, EWSR1, EZH2, FAM46C, FANCA, FANCC, FANCD2, FANCE, FANCF, FANCG, FANCL, FAS, FAT1, FBXW7, FGF10, FGF14, FGF19, FGF23, FGF3, FGF4, FGF6, FGFR1, FGFR2, FGFR3, FGFR4, FH, FLCN, FLI1, FLT1, FLT3, FLT4, FOLH1, FOXL2, FOXP1, FRS2, FUBP1, GABRA6, GATA1, GATA2, GATA3, GATA4, GATA6, GID4, GLI1, GNA11, GNA13, GNAQ, GNAS, GPR124, GRIN2A, GRM3, GSK3B, H3F3A, HAVCR2, HGF, HMGB1, HMGB2, HMGB3, HNF1A, HRAS, HSD3B1, HSP90AA1, IDHL IDH2, IDO, IGF1R, IGF2, IKBKE, IKZF1, IL7R, INHBA, INPP4B, IRF2, IRF4, IRS2, JAK1, JAK2, JAK3, JUN, MYST3, KDM5A, KDM5C, KDM6A, KDR, KEAP, KEL, KIT, KLHL6, KLK3, MLL, MLL2, MLL3, KRAS, LAG3, LMO1, LRP1B, LYN, LZTR1, MAGI2, MAP2K1, MAP2K2, MAP2K4, MAP3K1, MCL1, MDM2, MDM4, MED12, MEF2B, MEN1, MET, MITF, MLH1, MPL, MRE11A, MSH2, MSH6, MTOR, MUC1, MUTYH, MYC, MYCL, MYCN, MYD88, MYH, NF1, NF2, NFE2L2, NFKB1A, NKX2-1, NOTCH1, NOTCH2, NOTCH3, NPM1, NRAS, NSD1, NTRK1, NTRK2, NTRK3, NUP93, PAK3, PALB2, PARK2, PAX3, PAX, PBRM1, PDGFRA, PDCD1, PDCD1LG2, PDGFRB, PDK1, PGR, PIK3C2B, PIK3CA, PIK3CB, PIK3CG, PIK3R1, PIK3R2, PLCG2, PMS2, POLD1, POLE, PPP2R1A, PREX2, PRKAR1A, PRKC1, PRKDC, PRSS8, PTCH1, PTEN, PTPN11, QK1, RAC1, RAD50, RAD51, RAF 1, RANBP1, RARA, RB1, RBM10, RET, RICTOR, RIT1, RNF43, ROS1, RPTOR, RUNX1, RUNX1T1, SDHA, SDHB, SDHC, SDHD, SETD2, SF3B1, SLIT2, SMAD2, SMAD3, SMAD4, SMARCA4, SMARCB1, SMO, SNCAIP, SOCS1, SOX10, SOX2, SOX9, SPEN, SPOP, SPTA1, SRC, STAG2, STAT3, STAT4, STK11, SUFU, SYK, T (BRACHYURY), TAF1, TBX3, TERC, TERT, TET2, TGFRB2, TNFAIP3, TNFRSF14, TOP1, TOP2A, TP53, TSC1, TSC2, TSHR, U2AF1, VEGFA, VHL, WISP3, WT1, XPO1, ZBTB2, ZNF217, ZNF703, CD26, CD49F, CD44, CD49F, CD13, CD15, CD29, CD151, CD138, CD166, CD133, CD45, CD90, CD24, CD44, CD38, CD47, CD96, CD45, CD90, ABCB5, ABCG2, ALCAM, ALPHA-FETOPROTEIN, DLL1, DLL3, DLL4, ENDOGLIN, GJA1, OVASTACIN, AMACR, NESTIN, STRO-1, MICL, ALDH, BMI-1, GLI-2, CXCR1, CXCR2, CX3CR1, CX3CL1, CXCR4, PON1, TROP1, LGR5, MSI-1, C-MAF, TNFRSF7, TNFRSF16, SOX2, PODOPLANIN, L1CAM, HIF-2 ALPHA, TFRC, ERCC1, TUBB3, TOP1, TOP2A, TOP2B, ENOX2, TYMP, TYMS, FOLR1, GPNMB, PAPPA, GART, EBNA1, EBNA2, LMP1, BAGE, BAGE2, BCMA, C10ORF54, CD4, CD8, CD19, CD20, CD25, CD30, CD33, CD80, CD86, CD123, CD276, CCL1, CCL2, CCL3, CCL4, CCL5, CCL7, CCL8, CCL11, CCL13, CCL14, CCL15, CCL16, CCL17, CCL18, CCL19, CCL20, CCL21, CCL22, CCL23, CCL24, CCL25, CCL26, CCL27, CCL28, CCR1, CCR2, CCR3, CCR4, CCR5, CCR6, CCR7, CCR8, CCR9, CCR10, CXCL1, CXCL2, CXCL3, CXCL5, CXCL6, CXCL9, CXCL10, CXCL11, CXCL12, CXCL13, CXCL14, CXCL16, CXCL17, CXCR3, CXCR5, CXCR6, CTAG1B, CTAG2, CTAG1, CTAG4, CTAG5, CTAG6, CTAG9, CAGE1, GAGE1, GAGE2A, GAGE2B, GAGE2C, GAGE2D, GAGE2E, GAGE4, GAGE10, GAGE12D, GAGE12F, GAGE12J, GAGE13, HHLA2, ICOSLG, LAG1, MAGEA10, MAGEA12, MAGEA1, MAGEA2, MAGEA3, MAGEA4, MAGEA4, MAGEA5, MAGEA6, MAGEA7, MAGEA8, MAGEA9, MAGEB1, MAGEB2, MAGEB3, MAGEB4, MAGEB6, MAGEB10, MAGEB16, MAGEB18, MAGEC1, MAGEC2, MAGEC3, MAGED1, MAGED2, MAGED4, MAGED4B, MAGEE1, MAGEE2, MAGEF1, MAGEH1, MAGEL2, NCR3LG1, SLAMF7, SPAG1, SPAG4, SPAG5, SPAG6, SPAG7, SPAG8, SPAG9, SPAG11A, SPAG11B, SPAG16, SPAG17, VTCN1, XAGE1D, XAGE2, XAGE3, XAGE5, XCL1, XCL2, and XCR1. Of course, it should be appreciated that the above genes may be wild type or mutated versions, including missense or nonsense mutations, insertions, deletions, fusions, and/or translocations, all of which may or may not cause formation of full-length mRNA when transcribed.

[0032]For another example, some cell free DNAs/mRNAs are fragments of or those encoding a full length or a fragment of inflammation-related proteins, including, but not limited to, HMGB1, HMGB2, HMGB3, MUC1, VWF, MMP, CRP, PBEF1, TNF-α, TGF-β, PDGFA, IL-1, IL-2, IL-3, IL-4, IL-5, IL-6, IL-7, IL-8, IL-9, IL-10, IL-12, IL-13, IL-15, IL-17, Eotaxin, FGF, G-CSF, GM-CSF, IFN-γ, IP-10, MCP-1, PDGF, and hTERT, and in yet another example, the cell free mRNA encoded a full length or a fragment of HMGB1.

[0033]For still another example, some cell free DNAs/mRNAs are fragments of or those encoding a full length or a fragment of DNA repair-related proteins or RNA repair-related proteins. Table 1 provides an exemplary collection of predominant RNA repair genes and their associated repair pathways contemplated herein, but it should be recognized that numerous other genes associated with DNA repair and repair pathways are also expressly contemplated herein, and Tables 2 and 3 illustrate further exemplary genes for analysis and their associated function in DNA repair.

TABLE 1
Repair
mechanismPredominant DNA Repair genes
Base excisionDNA glycosylase, APE1, XRCC1, PNKP,
repair (BER)Tdp1, APTX, DNA polymerase β, FEN1,
DNA polymerase δ or ϵ, PCNA-RFC, PARP
MismatchMutSα (MSH2-MSH6), MutSβ (MSH2-
repair (MMR)MSH3), MutLα (MLH1-PMS2), MutLβ
(MLH1-PMS2), MutLγ (MLH1-MLH3),
Exo1, PCNA-RFC
NucleotideXPC-Rad23B-CEN2, UV-DDB (DDB1-XPE),
excision repairCSA, CSB, TFIIH, XPB, XPD, XPA, RPA,
(NER)XPG, ERCC1- XPF, DNA polymerase δ or ϵ
HomologousMre11-Rad50-Nbs1, CtIP, RPA, Rad51,
recombinationRad52, BRCA1, BRCA2, Exo1, BLM-TopIIIα,
(HR)GEN1-Yen1, Slx1- Slx4, Mus81/Eme1
Non-homologousKu70-Ku80, DNA-PKc, XRCC4-DNA ligase
end-joiningIV, XLF
(NHEJ)
TABLE 2
Gene nameAccession
(synonyms)Activitynumber
Base excision
repair (BER)
DNA glycosylases: major
altered base released
UNGU excisionNM_003362
SMUG1U excisionNM_014311
MBD4U or T opposite G at CpG sequencesNM_003925
TDGU, T or ethenoC opposite GNM_003211
OGG18-oxoG opposite CNM_002542
MYHA opposite 8-oxoGNM_012222
NTH1Ring-saturated or fragmentedNM_002528
pyrimidines
MPG3-meA, ethenoA, hypoxanthineNM_002434
Other BER factors
APE1 (HAP1,AP endonucleaseNM_001641
APEX, REF1)
APE2 (APEXL2)AP endonucleaseNM_014481
LIG3Main ligation functionNM_013975
XRCC1Main ligation functionNM_006297
Poly(ADP-ribose) polymerase
(PARP) enzymes
ADPRTProtects strand interruptionsNM_001618
ADPRTL2PARP-like enzymeNM_005485
ADPRTL3PARP-like enzymeAF085734
Direct reversal
of damage
MGMTO6-meG alkyltransferaseNM_002412
Mismatch excision
repair (MMR)
MSH2Mismatch and loop recognitionNM_000251
MSH3Mismatch and loop recognitionNM_002439
MSH6Mismatch recognitionNM_000179
MSH4MutS homolog specialized for meiosisNM_002440
MSH5MutS homolog specialized for meiosisNM_002441
PMS1Mitochondrial MutL homologNM_000534
MLH1MutL homologNM_000249
PMS2MutL homologNM_000535
MLH3MutL homolog of unknown functionNM_014381
PMS2L3MutL homolog of unknown functionD38437
PMS2L4MutL homolog of unknown functionD38438
Nucleotide excision
repair (NER)
XPCBinds damaged DNA as complexNM_004628
RAD23B (HR23B)Binds damaged DNA as complexNM_002874
CETN2Binds damaged DNA as complexNM_004344
RAD23A (HR23A)Substitutes for HR23BNM_005053
XPABinds damaged DNA in preincisionNM_000380
complex
RPA1Binds DNA in preincision complexNM_002945
RPA2Binds DNA in preincision complexNM_002946
RPA3Binds DNA in preincision complexNM_002947
TFIIHCatalyzes unwinding in preincision
complex
XPB (ERCC3)3′ to 5′ DNA helicaseNM_000122
XPD (ERCC2)5′ to 3′ DNA helicaseX52221
GTF2H1Core TFIIH subunit p62NM_005316
GTF2H2Core TFIIH subunit p44NM_001515
GTF2H3Core TFIIH subunit p34NM_001516
GTF2H4Core TFIIH subunit p52NM_001517
CDK7Kinase subunit of TFIIHNM_001799
CCNHKinase subunit of TFIIHNM_001239
MNAT1Kinase subunit of TFIIHNM_002431
XPG (ERCC5)3′ incisionNM_000123
ERCC15′ incision subunitNM_001983
XPF (ERCC4)5′ incision subunitNM_005236
LIG1DNA joiningNM_000234
NER-related
CSA (CKN1)Cockayne syndrome; needed forNM_000082
transcription-coupled NER
CSB (ERCC6)Cockayne syndrome; needed forNM_000124
transcription-coupled NER
XAB2 (HCNP)Cockayne syndrome; needed forNM_020196
transcription-coupled NER
DDB1Complex defective in XP group ENM_001923
DDB2Mutated in XP group ENM_000107
MMS19Transcription and NERAW852889
Homologous
recombination
RAD51Homologous pairingNM_002875
RAD51L1Rad51 homologU84138
(RAD51B)
RAD51CRad51 homologNM_002876
RAD51L3Rad51 homologNM_002878
(RAD51D)
DMC1Rad51 homolog, meiosisNM_007068
XRCC2DNA break and cross-link repairNM_005431
XRCC3DNA break and cross-link repairNM_005432
RAD52Accessory factor for recombinationNM_002879
RAD54LAccessory factor for recombinationNM_003579
RAD54BAccessory factor for recombinationNM_012415
BRCA1Accessory factor for transcriptionNM_007295
and recombination
BRCA2Cooperation with RAD51, essentialNM_000059
function
RAD50ATPase in complex with MRE11A,NM_005732
NBS1
MRE11A3′ exonucleaseNM_005590
NBS1Mutated in Nijmegen breakageNM_002485
syndrome
Nonhomologous
end-joining
Ku70 (G22P1)DNA end bindingNM_001469
Ku80 (XRCC5)DNA end bindingM30938
PRKDCDNA-dependent protein kinaseNM_006904
catalytic subunit
LIG4Nonhomologous end-joiningNM_002312
XRCC4Nonhomologous end-joiningNM_003401
Sanitization of
nucleotide pools
MTH1 (NUDT1)8-oxoGTPaseNM_002452
DUTdUTPaseNM_001948
DNA polymerases
(catalytic subunits)
POLBBER in nuclear DNANM_002690
POLGBER in mitochondrial DNANM_002693
POLD1NER and MMRNM_002691
POLE1NER and MMRNM_006231
PCNASliding clamp for pol delta and polNM_002592
epsilon
REV3L (POLZ)DNA pol zeta catalytic subunit,NM_002912
essential function
REV7 (MAD2L2)DNA pol zeta subunitNM_006341
REV1dCMP transferaseNM_016316
POLHXP variantNM_006502
POLI (RAD30B)Lesion bypassNM_007195
POLQDNA cross-link repairNM_006596
DINB1 (POLK)Lesion bypassNM_016218
POLLMeiotic functionNM_013274
POLMPresumed specialized lymphoidNM_013284
function
TRF4-1Sister-chromatid cohesionAF089896
TRF4-2Sister-chromatid cohesionAF089897
Editing and
processing
nucleases
FEN1 (DNase IV)5′ nucleaseNM_004111
TREX1 (DNase III)3′ exonucleaseNM_007248
TREX23′ exonucleaseNM_007205
EX01 (HEX1)5′ exonucleaseNM_003686
SPO11endonucleaseNM_012444
Rad6 pathway
UBE2A (RAD6A)Ubiquitin-conjugating enzymeNM_003336
UBE2B (RAD6B)Ubiquitin-conjugating enzymeNM_003337
RAD18Assists repair or replication ofAB035274
damaged DNA
UBE2VE (MMS2)Ubiquitin-conjugating complexAF049140
UBE2N (UBC13,Ubiquitin-conjugating complexNM_003348
BTG1)
Genes defective
in diseases
associated with
sensitivity to DNA
damaging agents
BLMBloom syndrome helicaseNM_000057
WRNWerner syndrome helicase/3′-NM_000553
exonuclease
RECQL4Rothmund-Thompson syndromeNM_004260
ATMAtaxia telangiectasiaNM_000051
Fanconi anemia
FANCAInvolved in tolerance or repairNM_000135
of DNA cross-links
FANCBInvolved in tolerance or repairN/A
of DNA cross-links
FANCCInvolved in tolerance or repairNM_000136
of DNA cross-links
FANCDInvolved in tolerance or repairN/A
of DNA cross-links
FANCEInvolved in tolerance or repairNM_021922
of DNA cross-links
FANCFInvolved in tolerance or repairAF181994
of DNA cross-links
FANCG (XRCC9)Involved in tolerance or repairNM_004629
of DNA cross-links
Other identified
genes with a
suspected DNA
repair function
SNM1 (PS02)DNA cross-link repairD42045
SNM1BRelated to SNM1AL137856
SNMICRelated to SNM1AA315885
RPA4Similar to RPA2NM_013347
ABH (ALKB)Resistance to alkylation damageX91992
PNKPConverts some DNA breaks toNM_007254
ligatable ends
Other conserved
DNA damage
response genes
ATRATM-and PI-3K-like essential kinaseNM_001184
RADI (S. pombe)PCNA-like DNA damage sensorNM_002853
homolog
RAD9 (S. pombe)PCNA-like DNA damage sensorNM_004584
homolog
HUS1 (S. pombe)PCNA-like DNA damage sensorNM_004507
homolog
RAD17 (RAD24)RFC-like DNA damage sensorNM_002873
TP53BP1BRCT proteinNM_005657
CHEK1Effector kinaseNM_001274
CHK2 (Rad53)Effector kinaseNM_007194
TABLE 3
Gene
NameGene TitleBiological Activity
RFC2replication factorDNA replication
C (activator 1)
2, 40 kDa
XRCC6X-ray repairDNA ligation///DNA repair///double-strand
complementingbreak repair via nonhomologous end-
defective repairjoining///DNA recombination///positive
in Chineseregulation of transcription, DNA-
hamsterdependent///double-strand break
cells 6 (Kurepair via nonhomologous
autoantigen,end-joining///response to DNA damage
70 kDa)stimulus///DNA recombination
APOBECapolipoprotein BFor all of APOBEC1, APOBEC2,
mRNA editingAPOBEC3A-H, and APOBEC4, cytidine
enzyme, catalyticdeaminases.
polypeptide-like
POLD2polymeraseDNA replication///DNA replication
(DNA directed),
delta 2,
regulatory sub-
unit 50 kDa
PCNAproliferating cellregulation of progression through cell
nuclear antigencycle///DNA replication///regulation of
DNA replication///DNA repair///cell
proliferation///phosphoinositide-mediated
signaling///DNA replication
RPA1replicationDNA-dependent DNA replication///DNA
protein A1,repair///DNA recombination///DNA
70 kDareplication
RPA1replicationDNA-dependent DNA replication///DNA
protein A1,repair///DNA recombination///
70 kDaDNA replication
RPA2replicationDNA replication///DNA-dependent DNA
protein A2,replication
32 kDa
ERCC3excision repairDNA topological change///
cross-transcription-coupled nucleotide-
complementingexcision repair///transcription///
rodentregulation of transcription,
repair deficiency,DNA-dependent///
complementationtranscription from RNA polymerase
group 3II promoter///induction of apoptosis///
(xerodermasensory perception of sound///
pigmentosumDNA repair///nucleotide-excision
group Brepair///response to DNA damage
complementing)stimulus///DNA repair
UNGuracil-DNAcarbohydrate metabolism///DNA
glycosylaserepair///base-excision repair///
response to DNA damage
stimulus///DNA repair///DNA repair
ERCC5excision repairtranscription-coupled nucleotide-
cross-excision repair///nucleotide-excision
complementingrepair///sensory perception of
rodentsound///DNA repair///response to DNA
repair deficiency,damage stimulus///nucleotide-
complementationexcision repair
group 5
(xeroderma
pigmentosum,
complementation
group G
(Cockayne
syndrome))
MLH1mutL homologmismatch repair///cell cycle///negative
1, colon cancer,regulation of progression through cell
nonpolyposiscycle///DNA repair///mismatch repair///
type 2 (<i>E.</i> <i>coli</i>)response to DNA damage stimulus
LIG1ligase I, DNA,DNA replication///DNA repair///DNA
ATP-dependentrecombination///cell cycle///
morphogenesis///cell division///DNA
repair///response to DNA damage
stimulus///DNA metabolism
NBNnibrinDNA damage checkpoint///cell cycle
checkpoint///double-strand break repair
NBNnibrinDNA damage checkpoint///cell cycle
checkpoint///double-strand break repair
NBNnibrinDNA damage checkpoint///cell cycle
checkpoint///double-strand break repair
MSH6mutS homolog 6mismatch repair///DNA metabolism///DNA
(<i>E.</i> <i>coli</i>)repair///mismatch repair///response to
DNA damage stimulus
POLD4polymeraseDNA replication///DNA replication
(DNA-directed),
delta 4
RFC5replicationDNA replication///DNA repair///DNA
factorreplication
C (activator
1) 5, 36.5 kDa
RFC5replication factorDNA replication///DNA repair///DNA
C (activator 1) 5,replication
36.5 kDa
DDB2///damage-specificnucleotide-excision repair///regulation of
LHX3DNA bindingtranscription, DNA-dependent///organ
protein 2, 48morphogenesis///DNA repair///response to
kDa///LIMDNA damage stimulus///DNA repair///
homeobox 3transcription///regulation of transcription
POLD1polymeraseDNA replication///DNA repair///response
(DNA directed),to UV///DNA replication
delta 1,
catalytic subunit
125 kDa
FANCGFanconi anemia,cell cycle checkpoint///DNA repair///DNA
complementationrepair///response to DNA damage
group Gstimulus///regulation of progression
through cell cycle
POLBpolymeraseDNA-dependent DNA replication///DNA
(DNA directed),repair///DNA replication///DNA repair///
betaresponse to DNA damage stimulus
XRCC1X-ray repairsingle strand break repair
complementing
defectivere pair
in Chinese
hamster cells 1
MPGN-methylpurine-base-excision repair///DNA dealkylation///
DNADNA repair///base-excision repair///
glycosylaseresponse to DNA damage stimulus
RFC2replication factorDNA replication
C (activator 1)
2, 40 kDa
ERCC1excision repairnucleotide-excision repair///
cross-morphogenesis///nucleotide-excision
complementingrepair///DNA repair///response to DNA
rodent repairdamage stimulus
deficiency,
complementation
group 1 (includes
overlapping
antisense
sequence)
TDGthymine-DNAcarbohydrate metabolism///base-excision
glycosylaserepair///DNA repair///response to
DNA damage stimulus
TDGthymine-DNAcarbohydrate metabolism///base-excision
glycosylaserepair///DNA repair///response to DNA
damage stimulus
FANCAFanconi anemia,DNA repair///protein complex assembly///
complementationDNA repair///response to DNA damage
group A///stimulus
Fanconi anemia,
complementation
group A
RFC4replication factorDNA replication///DNA strand elongation///
C (activator 1)DNA repair///phosphoinositide-mediated
4, 37 kDasignaling///DNA replication
RFC3replication factorDNA replication///DNA strand elongation
C (activator 1)
3, 38 kDa
RFC3replication factorDNA replication///DNA strand elongation
C (activator 1)
3, 38 kDa
APEX2APEX nucleaseDNA repair///response to DNA damage
(apurinic/stimulus
apyrimidinic
endonuclease) 2
RAD1RAD1 homologDNA repair///cell cycle checkpoint///cell
(S. pombe)cycle checkpoint///DNA damage check-
point///DNA repair///response to DNA
damage stimulus///meiotic prophase I
RAD1RAD1 homologDNA repair///cell cycle checkpoint///
(S. pombe)cell cycle checkpoint///DNA damage
checkpoint///DNA repair///response to
DNA damage stimulus///meiotic
prophase I
BRCA1breast cancer 1,regulation of transcription from RNA
early onsetpolymerase II promoter///regulation of
transcription from RNA polymerase III
promoter///DNA damage response, signal
transduction by p53 class mediator
resulting in transcription of p21 class
mediator///cell cycle///protein
ubiquitination///androgen receptor
signaling pathway///regulation of cell
proliferation///regulation of apoptosis///
positive regulation of DNA repair///
negative regulation of progression
through cell cycle///positive regulation
of transcription, DNA-dependent///
negative regulation of centriole
replication///DNA damage response,
signal transduction resulting in induction
of apoptosis///DNA repair///response
to DNA damage stimulus///protein
ubiquitination///DNA repair///regulation
of DNA repair///apoptosis///response
to DNA damage stimulus
EXO1exonuclease 1DNA repair///DNA repair///
mismatch repair///DNA recombination
FEN1flap structure-DNA replication///double-strand break
specificrepair///UV protection///phosphoinositide-
endonuclease 1mediated signaling///DNA repair///DNA
replication///DNA repair///DNA repair
FEN1flap structure-DNA replication///double-strand break
specificrepair///UV protection///phosphoinositide-
endonuclease 1mediated signaling///DNA repair///DNA
replication///DNA repair///DNA repair
MLH3mutL homolog 3mismatch repair///meiotic recombination///
(<i>E.</i> <i>coli</i>)DNA repair///mismatch repair///response to
DNA damage stimulus///mismatch repair
MGMTO-6-methyl-DNA ligation///DNA repair///response to
guanine-DNADNA damage stimulus
methyltransferase
RAD51RAD51 homologdouble-strand break repair via homologous
(RecA homolog,recombination///DNA unwinding during
replication///DNA repair///mitotic
(S. cerevisiae)recombination///meiosis///meiotic
recombination///positive regulation of DNA
ligation///protein homooligomerization///
response to DNA damage stimulus///DNA
metabolism///DNA repair///response to
DNA damage stimulus///DNA repair///
DNA recombination///meiotic
recombination///double-strand break repair
via homologous recombination///DNA
unwinding during replication
RAD51RAD51 homologdouble-strand break repair via homologous
(RecArecombination///DNA unwinding during
homolog, <i>E</i>. <i>coli</i>)replication///DNA repair///mitotic
(S. cerevisiae)recombination///meiosis///meiotic
recombination///positive regulation of DNA
ligation///protein homooligomerization///
response to DNA damage stimulus///DNA
metabolism///DNA repair///response to
DNA damage stimulus///DNA repair///DNA
recombination///meiotic recombination///
double-strand break repair via homologous
recombination///DNA unwinding during
replication
XRCC4X-ray repairDNA repair///double-strand break repair///
complementingDNA recombination///DNA
defective repair inrecombination///response to DNA damage
Chinese hamsterstimulus
cells 4
XRCC4X-ray repairDNA repair///double-strand break repair///
complementingDNA recombination///DNA
defective repair inrecombination///response to DNA
Chinese hamsterdamage stimulus
cells 4
RECQLRecQ protein-DNA repair///DNA metabolism
like (DNA
helicase Q1-like)
ERCC8excision repairDNA repair///transcription///regulation of
cross-transcription, DNA-dependent///sensory
complementingperception of sound///transcription-
rodent repaircoupled nucleotide-excision repair
deficiency,
complementation
group 8
FANCCFanconi anemia,DNA repair///DNA repair///protein
complementationcomplex assembly///response to DNA
group Cdamage stimulus
OGG18-oxoguaninecarbohydrate metabolism///base-excision
DNArepair///DNA repair///base-excision
glycosylaserepair///response to DNA
damage stimulus///DNA repair
MRE11AMRE11 meioticregulation of mitotic recombination///
recombinationdouble-strand break repair via
11 homolog Anonhomologous end-
(S. cerevisiae)joining///telomerase-dependent telomere
maintenance///meiosis///meiotic
recombination///DNA metabolism///
DNA repair///double-strand break repair///
response to DNA damage stimulus///
DNA repair///double-strand break repair///
DNA recombination
RAD52RAD52 homologdouble-strand break repair///mitotic
(S. cerevisiae)recombination///meiotic recombination///
DNA repair///DNA recombination///
response to DNA damage stimulus
WRNWerner syndromeDNA metabolism///aging
XPAxerodermanucleotide-excision repair///DNA repair///
pigmentosum,response to DNA damage stimulus///DNA
complementationrepair///nucleotide-excision repair
group A
BLMBloom syndromeDNA replication///DNA repair///DNA
recombination///antimicrobial humoral
response (sensu Vertebrata)///DNA
metabolism///DNA replication
OGG18-oxoguaninecarbohydrate metabolism///base-excision
DNArepair///DNA repair///base-excision
glycosylaserepair///response to DNA damage
stimulus///DNA repair
MSH3mutS homolog 3mismatch repair///DNA metabolism///DNA
(<i>E.</i> <i>coli</i>)repair///mismatch repair///response to
DNA damage stimulus
POLE2polymerase (DNADNA replication///DNA repair///DNA
directed), epsilonreplication
2 (p59 subunit)
RAD51CRAD51 homologDNA repair///DNA recombination///DNA
C (<i>S.</i> <i>cerevisiae</i>)metabolism///DNA repair///DNA
recombination///response to DNA
damage stimulus
LIG4ligase IV, DNA,single strand break repair///DNA
ATP-dependentreplication///DNA recombination///cell
cycle///cell division///DNA repair///
response to DNA damage stimulus
ERCC6excision repairDNA repair///transcription///regulation of
cross-transcription, DNA-dependent///
complementingtranscription from RNA
rodent repairpolymerase II promoter///sensory
deficiency,perception of sound
complementation
group 6
LIG3ligase III, DNA,DNA replication///DNA repair///cell cycle///
ATP-dependentmeiotic recombination///spermatogenesis///
cell division///DNA repair///
DNA recombination///response to
DNA damage stimulus
RAD17RAD17 homologDNA replication///DNA repair///cell cycle///
(S. pombe)response to DNA damage stimulus
XRCC2X-ray repairDNA repair///DNA recombination///
complementingmeiosis///DNA metabolism///DNA repair///
defective repair inresponse to DNA damage stimulus
Chinese hamster
cells 2
MUTYHmutY homologcarbohydrate metabolism///base-excision
(<i>E.</i> <i>coli</i>)repair///mismatch repair///cell cycle///
negative regulation of progression
through cell cycle///DNA repair///response
to DNA damage stimulus///DNA repair
RFC1replication factorDNA-dependent DNA replication///
C (activator 1) 1,transcription///regulation of transcription,
145 kDa///DNA-dependent///telomerase-dependent
replication factortelomere maintenance///DNA
C (activator 1) 1,replication///DNA repair
145 kDa
RFC1replication factorDNA-dependent DNA replication///
C (activator 1) 1,transcription///regulation of transcription,
145 kDaDNA-dependent///telomerase-
dependent telomere maintenance///
DNA replication///DNA repair
BRCA2breast cancer 2,regulation of progression through cell
early onsetcycle///double-strand break repair via
homologous recombination///DNA
repair///establishment and/or
maintenance of chromatin architecture///
chromatin remodeling///regulation of
S phase of mitotic cell
cycle///mitotic checkpoint///regulation of
transcription///response to DNA damage
stimulus
RAD50RAD50 homologregulation of mitotic recombination///
(S. cerevisiae)double-strand break repair///telomerase-
dependent telomere maintenance///
cell cycle///meiosis///meiotic
recombination///chromosome
organization and biogenesis///telomere
maintenance///DNA repair///response
to DNA damage stimulus///DNA
repair///DNA recombination
DDB1damage-specificnucleotide-excision repair///ubiquitin
DNA bindingcycle///DNA repair///response to DNA
protein 1,damage stimulus///DNA repair
127 kDa
XRCC5X-ray repairdouble-strand break repair via
complementingnonhomologous end-joining///DNA
defective repairrecombination///DNA repair///
in ChineseDNA recombination///response to
hamsterDNA damage stimulus///double-strand
cells 5 (double-break repair
strand-break
rejoining;
Ku autoantigen,
80 kDa)
XRCC5X-ray repairdouble-strand break repair via non-
complementinghomologous end-joining///DNA
defective repairrecombination///DNA repair///
in ChineseDNA recombination///response to DNA
hamsterdamage stimulus///double-strand break
cells 5 (double-repair
strand-break
rejoining; Ku
autoantigen,
80 kDa)
PARP1poly (ADP-ribose)DNA repair///transcription from RNA
polymerasepolymerase II promoter///protein amino
family,acid ADP-ribosylation///DNA
member 1metabolism///DNA repair///protein
amino acid ADP-ribosylation///
response to DNA damage stimulus
POLE3polymerase (DNADNA replication
directed), epsilon
3 (p17 subunit)
RFC1replication factorDNA-dependent DNA replication///
C (activator 1) 1,transcription///regulation of transcription,
145 kDaDNA-dependent///telomerase-
dependent telomere maintenance///
DNA replication///DNA repair
RAD50RAD50 homologregulation of mitotic recombination///
(S. cerevisiae)double-strand break repair///
telomerase-dependent telomere
maintenance///cell cycle///meiosis///
meiotic recombination///chromosome
organization and biogenesis///telomere
maintenance///DNA repair///response
to DNA damage stimulus///DNA
repair///DNA recombination
XPCxerodermanucleotide-excision repair///DNA repair///
pigmentosum,nucleotide-excision repair///response to
complementationDNA damage stimulus///DNA repair
group C
MSH2mutS homolog 2,mismatch repair///postreplication repair///
colon cancer,cell cycle///negative regulation
nonpolyposisof progression through cell cycle///
type 1 (<i>E.</i> <i>coli</i>)DNA metabolism///DNA
repair///mismatch repair///response to
DNA damage stimulus///DNA repair
RPA3replicationDNA replication///DNA repair///DNA
protein
A3, 14 kDa
MBD4methyl-replication base-excision repair///DNA
CpG bindingrepair///response to DNA damage
domainstimulus///DNA repair
protein 4
MBD4methyl-CpGbase-excision repair///DNA repair///
binding domainresponse to DNA damage stimulus///
protein 4DNA repair
NTHL1nth endonucleasecarbohydrate metabolism///base-excision
III-like 1repair///nucleotide-excision repair, DNA
(<i>E.</i> <i>coli</i>)incision, 5′-to lesion///DNA repair///
response to DNA damage stimulus
PMS2///PMS2mismatch repair///cell cycle///negative
PMS2CLpostmeioticregulation of progression through cell
segregationcycle///DNA repair///mismatch
increased 2 (S.repair///response to DNA damage
cerevisiae)///stimulus///mismatch repair
PMS2-C
terminal-like
RAD51CRAD51 homologDNA repair///DNA recombination///DNA
C (S. cerevisiae)metabolism///DNA repair///DNA
recombination///response to DNA damage
stimulus
UNG2uracil-DNAregulation of progression through cell
glycosylase 2cycle///carbohydrate metabolism///base-
excision repair///DNA repair///response to
DNA damage stimulus
APEX1APEX nucleasebase-excision repair///transcription from
(multifunctionalRNA polymerase II promoter///regulation
DNA repairof DNA binding///DNA repair///
enzyme) 1response to DNA damage stimulus
ERCC4excision repairnucleotide-excision repair///nucleotide-
cross-excision repair///DNA metabolism///DNA
complementingrepair///response to DNA damage stimulus
rodent repair
deficiency,
complementation
group 4
RAD1RAD1 homologDNA repair///cell cycle checkpoint///
(S. pombe)cell cycle checkpoint///DNA damage
checkpoint///DNA repair///response to
DNA damage stimulus///
meiotic prophase I
RECQL5RecQ protein-DNA repair///DNA metabolism///DNA
like 5metabolism
MSH5mutS homolog 5DNA metabolism///mismatch repair///
(<i>E.</i> <i>coli</i>)mismatch repair///meiosis///meiotic
recombination///meiotic prophase II///
meiosis
RECQLRecQ protein-DNA repair///DNA metabolism
like (DNA
helicase Q1-like)
RAD52RAD52 homologdouble-strand break repair///mitotic
(S. cerevisiae)recombination///meiotic recombination///
DNA repair///DNA recombination///
response to DNA damage stimulus
XRCC4X-ray repairDNA repair///double-strand break repair///
complementingDNA recombination///DNA
defective repairrecombination///response to DNA
in Chinesedamage stimulus
hamster cells 4
XRCC4X-ray repairDNA repair///double-strand break repair///
complementingDNA recombination///DNA
defective repair inrecombination///response to DNA
Chinese hamsterdamage stimulus
cells 4
RAD17RAD17 homologDNA replication///DNA repair///cell
(S. pombe)cycle///response to DNA damage stimulus
MSH3mutS homologmismatch repair///
3 (<i>E.</i> <i>coli</i>)DNA metabolism///DNA repair///
mismatch repair///response to DNA
damage stimulus
MRE11AMRE11 meioticregulation of mitotic recombination///
recombination 11double-strand break repair via
homolog Anonhomologous end-joining///
(S. cerevisiae)telomerase-dependent telomere
maintenance///meiosis///meiotic
recombination///DNA metabolism///
DNA repair///double-strand break
repair///response to DNA damage
stimulus///DNA repair///double-strand
break repair///DNA recombination
MSH6mutS homolog 6mismatch repair///DNA metabolism///
(<i>E.</i> <i>coli</i>)DNA repair///mismatch repair///response
to DNA damage stimulus
MSH6mutS homolog 6mismatch repair///DNA metabolism///
(<i>E.</i> <i>coli</i>)DNA repair///mismatch repair///
response to DNA damage stimulus
RECQL5RecQ protein-DNA repair///DNA metabolism///DNA
like 5metabolism
BRCA1breast cancer 1,regulation of transcription from RNA
early onsetpolymerase II promoter///regulation of
transcription from RNA polymerase III
promoter///DNA damage response,
signal transduction by p53 class
mediator resultingi n transcription of
p21 class mediator///cell
cycle///protein ubiquitination///androgen
receptor signaling pathway///regulation
of cell proliferation///regulation of
apoptosis///positive regulation of DNA
repair///negative regulation of
progression through cell cycle///
positive regulation of transcription,
DNA-dependent///negative regulation of
centriole replication///DNA damage
response, signal transduction resulting
in induction of apoptosis///DNA repair///
response to DNA damage stimulus///
protein ubiquitination///DNA repair///
regulation of DNA repair///apoptosis///
response to DNA damage stimulus
RAD52RAD52 homologdouble-strand break repair///mitotic
(S. cerevisiae)recombination///meiotic recombination///
DNA repair///DNA recombination///
response to DNA damage stimulus
POLD3polymeraseDNA synthesis during DNA repair///
(DNA-directed),mismatch repair///DNA replication
delta
3, accessory
subunit
MSH5mutS homolog 5DNA metabolism///mismatch repair///
(<i>E.</i> <i>coli</i>)mismatch repair///meiosis///meiotic
recombination///meiotic
prophase II///meiosis
ERCC2excision repairtranscription-coupled nucleotide-
cross-excision repair///transcription///regulation
complementingof transcription, DNA-dependent///
rodent repairtranscription from RNA polymerase II
deficiency,promoter///induction of apoptosis///
complementationsensory perception of sound///
group 2nucleobase, nucleoside, nucleotide
(xerodermaand nucleic acid metabolism///
pigmentosum D)nucleotide-excision repair
RECQL4RecQ protein-DNA repair///development///DNA
like 4metabolism
PMS1PMS1mismatch repair///regulation of
postmeiotictranscription, DNA-dependent///cell
segregationcycle///negative regulation
increased 1of progression through cell
(S. cerevisiae)cycle///mismatch repair///DNA repair///
response to DNA damage stimulus
ZFP276zinc fingertranscription///regulation of transcription,
proteinDNA-dependent
276 homolog
(mouse)
MBD4methyl-CpGbase-excision repair///DNA repair///
binding domainresponse to DNA damage stimulus///
protein 4DNA repair
MBD4methyl-CpGbase-excision repair///DNA repair///
binding domainresponse to DNA damage stimulus///
protein 4DNA repair
MLH3mutL homolog 3mismatch repair///meiotic recombination///
(<i>E.</i> <i>coli</i>)DNA repair///mismatch repair///
response to DNA damage stimulus///
mismatch repair
FANCAFanconi anemia,DNA repair///protein complex assembly///
complementationDNA repair///response to DNA damage
group Astimulus
POLEpolymeraseDNA replication///DNA repair///DNA
(DNA directed),replication///response to DNA damage
epsilonstimulus
XRCC3X-ray repairDNA repair///DNA recombination///
complementingDNA metabolism///
defectiveDNA repair///DNA recombination///
repair in Chineseresponse to DNA damage stimulus///
hamster cells 3response to DNA damage stimulus
MLH3mutL homolog 3mismatch repair///meiotic recombination///
(<i>E.</i> <i>coli</i>)DNA repair///mismatch repair///
response to DNA damage stimulus///
mismatch repair
NBNnibrinDNA damage checkpoint///cell cycle
checkpoint///double-strand break repair
SMUG1single-strandcarbohydrate metabolism///DNA repair///
selectiveresponse to DNA damage stimulus
monofunctional
uracil DNA
glycosylase
FANCFFanconi anemia,DNA repair///response to DNA damage
complementationstimulus
group F
NEIL1nei endonucleasecarbohydrate metabolism///DNA repair///
VIII-like 1response to DNA damage stimulus
(<i>E.</i> <i>coli</i>)
FANCEFanconi anemia,DNA repair///response to DNA damage
complementationstimulus
group E
MSH5mutS homolog 5DNA metabolism///mismatch repair///
(<i>E.</i> <i>coli</i>)mismatch repair///meiosis///meiotic
recombination///meiotic prophase II///
meiosis
RECQL5RecQ protein-DNA repair///DNA metabolism///DNA
like 5metabolism

[0034]For still another example, some cell free DNAs/mRNAs are fragments of or those encoding a full length or a fragment of a gene not associated with a disease (e.g., housekeeping genes), including, but not limited to, those related to transcription factors (e.g., ATF1, ATF2, ATF4, ATF6, ATF7, ATFIP, BTF3, E2F4, ERH, HMGB1, ILF2, IER2, JUND, TCEB2, etc.), repressors (e.g., PUF60), RNA splicing (e.g., BAT1, HNRPD, HNRPK, PABPN1, SRSF3, etc.), translation factors (EIF1, EIF1AD, EIF1B, EIF2A, EIF2AK1, EIF2AK3, EIF2AK4, EIF2B2, EIF2B3, EIF2B4, EIF2S2, EIF3A, etc.), tRNA synthetases (e.g., AARS, CARS, DARS, FARS, GARS, HARS, IARS, KARS, MARS, etc.), RNA binding protein (e.g., ELAVL1, etc.), ribosomal proteins (e.g., RPL5, RPL8, RPL9, RPL10, RPL11, RPL14, RPL25, etc.), mitochondrial ribosomal proteins (e.g., MRPL9, MRPL1, MRPL10, MRPL11, MRPL12, MRPL13, MRPL14, etc.), RNA polymerase (e.g., POLR1C, POLR1D, POLR1E, POLR2A, POLR2B, POLR2C, POLR2D, POLR3C, etc.), protein processing (e.g., PPID, PPI3, PPIF, CANX, CAPN1, NACA, PFDN2, SNX2, SS41, SUM01, etc.), heat shock proteins (e.g., HSPA4, HSPA5, HSBP1, etc.), histone (e.g., HIST1HSBC, H1FX, etc.), cell cycle (e.g., ARHGAP35, RAB 10, RAB 11A, CCNY, CCNL, PPP1CA, RAD1, RAD17, etc.), carbohydrate metabolism (e.g., ALDOA, GSK3A, PGK1, PGAM5, etc.), lipid metabolism (e.g., HADHA), citric acid cycle (e.g., SDHA, SDHB, etc.), amino acid metabolism (e.g., COMT, etc.), NADH dehydrogenase (e.g., NDUFA2, etc.), cytochrome c oxidase (e.g., COX5B, COX8, COX11, etc.), ATPase (e.g. ATP2C1, ATP5F1, etc.), lysosome (e.g., CTSD, CSTB, LAMP1, etc.), proteasome (e.g., PSMA1, UBA1, etc.), cytoskeletal proteins (e.g., ANXA6, ARPC2, etc.), and organelle synthesis (e.g., BLOC1S1, AP2A1, etc.).

[0035]In still another example, some cell free DNAs/mRNAs are fragments of or those encoding a full length or a fragment of a neoepitope specific to the tumor. With respect to neoepitope, it should be appreciated that neoepitopes can be characterized as random mutations in tumor cells that create unique and tumor specific antigens. Therefore, high-throughput genome sequencing should allow for rapid and specific identification of patient specific neoepitopes where the analysis also considers matched normal tissue of the same patient. In some embodiments, neoepitopes may be identified from a patient tumor in a first step by whole genome analysis of a tumor biopsy (or lymph biopsy or biopsy of a metastatic site) and matched normal tissue (i.e., non-diseased tissue from the same patient) via synchronous comparison of the so obtained omics information. While not limiting to the inventive subject matter, it is typically preferred that the data are patient matched tumor data (e.g., tumor versus same patient normal), and that the data format is in SAM, BAM, GAR, or VCF format. However, non-matched or matched versus other reference (e.g., prior same patient normal or prior same patient tumor, or homo statisticus) are also deemed suitable for use herein. Therefore, the omics data may be ‘fresh’ omics data or omics data that were obtained from a prior procedure (or even different patient). However, and especially where genomics ctDNA is analyzed, the neoepitope-coding sequence need not necessarily be expressed.

[0036]In particularly preferred aspects, the nucleic acid encoding a neoepitope may encode a neoepitope that is also a suitable target for immune therapy. Therefore, neoepitopes can then be further filtered for a match to the patient's HLA type to thereby increase likelihood of antigen presentation of the neoepitope. Most preferably, and as further discussed below, such matching can be done in silico. Most typically, the patient-specific epitopes are unique to the patient, but may also in at least some cases include tumor type-specific neoepitopes (e.g., Her-2, PSA, brachyury) or cancer-associated neoepitopes (e.g., CEA, MUC-1, CYPB1).

[0037]It is contemplated that cell free DNA/mRNA may present in modified forms or different isoforms. For example, the cell free DNA may be present in methylated or hydroxyl methylated, and the methylation level of some genes (e.g., GSTP1, p16, APC, etc.) may be a hallmark of specific types of cancer (e.g., colorectal cancer, etc.). The cell free mRNA may be present in a plurality of isoforms (e.g., splicing variants, etc.) that may be associated with different cell types and/or location. Preferably, different isoforms of mRNA may be a hallmark of specific tissues (e.g., brain, intestine, adipose tissue, muscle, etc.), or may be a hallmark of cancer (e.g., different isoform is present in the cancer cell compared to corresponding normal cell, or the ratio of different isoforms is different in the cancer cell compared to corresponding normal cell, etc.). For example, mRNA encoding HMGB1 are present in 18 different alternative splicing variants and 2 unspliced forms. Those isoforms are expected to express in different tissues/locations of the patient's body (e.g., isoform A is specific to prostate, isoform B is specific to brain, isoform C is specific to spleen, etc.). Thus, in these embodiments, identifying the isoforms of cell free mRNA in the patient's bodily fluid can provide information on the origin (e.g., cell type, tissue type, etc.) of the cell free mRNA.

[0038]The inventors contemplate that the quantities and/or isoforms (or subtypes) or regulatory noncoding RNA (e.g., microRNA, small interfering RNA, long non-coding RNA (lncRNA)) can vary and fluctuate by presence of a tumor or immune response against the tumor. Without wishing to be bound by any specific theory, varied expression of regulatory noncoding RNA in a cancer patient's bodily fluid may due to genetic modification of the cancer cell (e.g., deletion, translocation of parts of a chromosome, etc.), and/or inflammations at the cancer tissue by immune system (e.g., regulation of miR-29 family by activation of interferon signaling and/or virus infection, etc.). Thus, in some embodiments, the cell free RNA can be a regulatory noncoding RNA that modulates expression (e.g., downregulates, silences, etc.) of mRNA encoding a cancer-related protein or an inflammation-related protein (e.g., HMGB1, HMGB2, HMGB3, MUC1, VWF, MMP, CRP, PBEF1, TNF-α, TGF-β, PDGFA, IL-1, IL-2, IL-3, IL-4, IL-5, IL-6, IL-7, IL-8, IL-9, IL-10, IL-12, IL-13, IL-15, IL-17, Eotaxin, FGF, G-CSF, GM-CSF, IFN-γ, IP-10, MCP-1, PDGF, hTERT, etc.).

[0039]It is also contemplated that some cell free regulatory noncoding RNA may be present in a plurality of isoforms or members (e.g., members of miR-29 family, etc.) that may be associated with different cell types and/or location. Preferably, different isoforms or members of regulatory noncoding RNA may be a hallmark of specific tissues (e.g., brain, intestine, adipose tissue, muscle, etc.), or may be a hallmark of cancer (e.g., different isoform is present in the cancer cell compared to corresponding normal cell, or the ratio of different isoforms is different in the cancer cell compared to corresponding normal cell, etc.). For example, higher expression level of miR-155 in the bodily fluid can be associated with the presence of breast tumor, and the reduced expression level of miR-155 can be associated with reduced size of breast tumor. Thus, in these embodiments, identifying the isoforms of cell free regulatory noncoding RNA in the patient's bodily fluid can provide information on the origin (e.g., cell type, tissue type, etc.) of the cell free regulatory noncoding RNA.

Isolation and Amplification of Cell Free DNA/RNA

[0040]Any suitable methods to isolate and amplify cell free DNA/RNA are contemplated. Most typically, cell free DNA/RNA is isolated from a bodily fluid (e.g., whole blood) that is processed under a suitable conditions, including a condition that stabilizes cell free RNA. Preferably, both cell free DNA and RNA are isolated simultaneously from the same badge of the patient's bodily fluid. Yet, it is also contemplated that the bodily fluid sample can be divided into two or more smaller samples from which DNA or RNA can be isolated separately. Once separated from the non-nucleic acid components, cell free RNA are then quantified, preferably using real time, quantitative PCR or real time, quantitative RT-PCR.

[0041]The bodily fluid of the patient can be obtained at any desired time point(s) depending on the purpose of the omics analysis. For example, the bodily fluid of the patient can be obtained before and/or after the patient is confirmed to have a tumor and/or periodically thereafter (e.g., every week, every month, etc.) in order to associate the cell free DNA/RNA data with the prognosis of the cancer. In some embodiments, the bodily fluid of the patient can be obtained from a patient before and after the cancer treatment (e.g., chemotherapy, radiotherapy, drug treatment, cancer immunotherapy, etc.). While it may vary depending on the type of treatments and/or the type of cancer, the bodily fluid of the patient can be obtained at least 24 hours, at least 3 days, at least 7 days after the cancer treatment. For more accurate comparison, the bodily fluid from the patient before the cancer treatment can be obtained less than 1 hour, less than 6 hours before, less than 24 hours before, less than a week before the beginning of the cancer treatment. In addition, a plurality of samples of the bodily fluid of the patient can be obtained during a period before and/or after the cancer treatment (e.g., once a day after 24 hours for 7 days, etc.).

[0042]Additionally or alternatively, the bodily fluid of a healthy individual can be obtained to compare the sequence/modification of cell free DNA, and/or quantity/subtype expression of cell free RNA. As used herein, a healthy individual refers an individual without a tumor. Preferably, the healthy individual can be chosen among group of people shares characteristics with the patient (e.g., age, gender, ethnicity, diet, living environment, family history, etc.).

[0043]Any suitable methods for isolating cell free DNA/RNA are contemplated. For example, in one exemplary method of DNA isolation, specimens were accepted as 10 ml of whole blood drawn into a test tube. Cell free DNA can be isolated from other from mono-nucleosomal and di-nucleosomal complexes using magnetic beads that can separate out cell free DNA at a size between 100-300 bps. For another example, in one exemplary method of RNA isolation, specimens were accepted as 10 ml of whole blood drawn into cell-free RNA BCT® tubes or cell-free DNA BCT® tubes containing RNA stabilizers, respectively. Advantageously, cell free RNA is stable in whole blood in the cell-free RNA BCT tubes for seven days while cell free RNA is stable in whole blood in the cell-free DNA BCT Tubes for fourteen days, allowing time for shipping of patient samples from world-wide locations without the degradation of cell free RNA. Moreover, it is generally preferred that the cell free RNA is isolated using RNA stabilization agents that will not or substantially not (e.g., equal or less than 1%, or equal or less than 0.1%, or equal or less than 0.01%, or equal or less than 0.001%) lyse blood cells. Viewed from a different perspective, the RNA stabilization reagents will not lead to a substantial increase (e.g., increase in total RNA no more than 10%, or no more than 5%, or no more than 2%, or no more than 1%) in RNA quantities in serum or plasma after the reagents are combined with blood. Likewise, these reagents will also preserve physical integrity of the cells in the blood to reduce or even eliminate release of cellular RNA found in blood cell. Such preservation may be in form of collected blood that may or may not have been separated. In less preferred aspects, contemplated reagents will stabilize cell free RNA in a collected tissue other than blood for at 2 days, more preferably at least 5 days, and most preferably at least 7 days. Of course, it should be recognized that numerous other collection modalities are also deemed appropriate, and that the cell free RNA can be at least partially purified or adsorbed to a solid phase to so increase stability prior to further processing.

[0044]As will be readily appreciated, fractionation of plasma and extraction of cell free DNA/RNA can be done in numerous manners. In one exemplary preferred aspect, whole blood in 10 mL tubes is centrifuged to fractionate plasma at 1600 rcf for 20 minutes. The so obtained plasma is then separated and centrifuged at 16,000 rcf for 10 minutes to remove cell debris. Of course, various alternative centrifugal protocols are also deemed suitable so long as the centrifugation will not lead to substantial cell lysis (e.g., lysis of no more than 1%, or no more than 0.1%, or no more than 0.01%, or no more than 0.001% of all cells). Cell free RNA is extracted from 2 mL of plasma using Qiagen reagents. The extraction protocol was designed to remove potential contaminating blood cells, other impurities, and maintain stability of the nucleic acids during the extraction. All nucleic acids were kept in bar-coded matrix storage tubes, with DNA stored at −4° C. and RNA stored at −80° C. or reverse-transcribed to cDNA that is then stored at −4° C. Notably, so isolated cell free RNA can be frozen prior to further processing.

Omics Data Processing

[0045]Once cell free DNA/RNA is isolated, various types of omics data can be obtained using any suitable methods. DNA sequence data will not only include the presence or absence of a gene that is associated with cancer or inflammation, but also take into account mutation data where the gene is mutated, the copy number (e.g., to identify duplication, loss of allele or heterozygosity), and epigenetic status (e.g., methylation, histone phosphorylation, nucleosome positioning, etc.). With respect to RNA sequence data it should be noted that contemplated RNA sequence data include mRNA sequence data, splice variant data, polyadenylation information, etc. Moreover, it is generally preferred that the RNA sequence data also include a metric for the transcription strength (e.g., number of transcripts of a damage repair gene per million total transcripts, number of transcripts of a damage repair gene per total number of transcripts for all damage repair genes, number of transcripts of a damage repair gene per number of transcripts for actin or other household gene RNA, etc.), and for the transcript stability (e.g., a length of poly A tail, etc.).

[0046]With respect to the transcription strength (expression level), transcription strength of the cell free RNA can be examined by quantifying the cell free RNA. Quantification of cell free RNA can be performed in numerous manners, however, expression of analytes is preferably measured by quantitative real-time RT-PCR of cell free RNA using primers specific for each gene. For example, amplification can be performed using an assay in a 10 μL reaction mix containing 2 μL cell free RNA, primers, and probe. mRNA of α-actin can be used as an internal control for the input level of cell free RNA. A standard curve of samples with known concentrations of each analyte was included in each PCR plate as well as positive and negative controls for each gene. Test samples were identified by scanning the 2D barcode on the matrix tubes containing the nucleic acids. Delta Ct (dCT) was calculated from the Ct value derived from quantitative PCR (qPCR) amplification for each analyte subtracted by the Ct value of actin for each individual patient's blood sample. Relative expression of patient specimens is calculated using a standard curve of delta Cts of serial dilutions of Universal Human Reference RNA set at a gene expression value of 10 (when the delta CTs were plotted against the log concentration of each analyte).

[0047]Alternatively, where discovery or scanning for new mutations or changes in expression of a particular gene is desired, real time quantitative PCR may be replaced by RNAseq to so cover at least part of a patient transcriptome. Moreover, it should be appreciated that analysis can be performed static or over a time course with repeated sampling to obtain a dynamic picture without the need for biopsy of the tumor or a metastasis.

[0048]Thus, omics data of cell free DNA/RNA preferably comprise a genomic data set that includes genomic sequence information. Most typically, the genomic sequence information comprises DNA sequence information of cell free DNA of the patient and optionally cell free DNA of a healthy individual. The sequence data sets may include unprocessed or processed data sets, and exemplary data sets include those having BAM format, SAM format, FASTQ format, or FASTA format. However, it is especially preferred that the data sets are provided in BAM format or as BAMBAM diff objects (see e.g., US2012/0059670A1 and US2012/0066001A1). Moreover, it should be noted that the data sets are reflective of the cell free DNA/RNA of the patient and of the healthy individual to so obtain patient and tumor specific information. Thus, genetic germ line alterations not giving rise to the diseased cells (e.g., silent mutation, SNP, etc.) can be excluded. Further, so obtained omics information can then be processed using pathway analysis (especially using PARADIGM) to identify any impact of any mutations on DNA repair pathways.

[0049]Likewise, computational analysis of the sequence data may be performed in numerous manners. In most preferred methods, however, analysis is performed in silico by location-guided synchronous alignment of cell free DNA/RNA of the patient and a healthy individual as, for example, disclosed in US 2012/0059670A1 and US 2012/0066001A1 using BAM files and BAM servers. Such analysis advantageously reduces false positive data and significantly reduces demands on memory and computational resources.

[0050]With respect to the analysis of cell free DNA/RNA of the patient and a healthy individual, numerous manners are deemed suitable for use herein so long as such methods will be able to generate a differential sequence object. However, it is especially preferred that the differential sequence object is generated by incremental synchronous alignment of BAM files representing genomic sequence information of the cell free DNA/RNA of the patient and a healthy individual. For example, particularly preferred methods include BAMBAM-based methods as described in US 2012/0059670 and US 2012/0066001.

Omics Data Analysis: Calculation of a Score

[0051]For calculation of a score, it should be appreciated that all data from ct/cf nucleic acids are deemed suitable for use herein and may therefore be specific to a particular tumor and/or patient and/or specific to a cancer. Furthermore, such data may be further normalized or otherwise preprocessed to adjust for age, treatment, gender, stage of disease, etc.

[0052]For example, in one aspect of the inventive subject matter the inventors contemplate that a library or reference base for all cancer-related genes, inflammation-related genes, DNA repair-related genes, and/or other non-disease related housekeeping genes can be created using one or more omics data for each of those genes, and such library is particularly useful where the omics data are associated with one or more health parameter. Viewed from a different perspective, while traditional methods of determining cancer prognosis or predicting treatment outcome have been based on a few number of genes, such library can provide a tool to generate a large cross-sectional database for all cancer-related gene activity, inflammation-related gene activity, DNA repair gene activity and housekeeping gene activity (as a control). The large cross-sectional database can be a basis for generating a cancer matrix, based on which a prognosis of a cancer, a health status of the patient, a likelihood of outcome of treatment, an effectiveness of the treatment can be more reliably calculated.

[0053]Of course, it should be appreciated that analyses presented herein may be performed over specific and diverse populations to so obtain reference values for the specific populations, such as across various health associated states (e.g., healthy, diagnosed with a specific disease and/or disease state, which may or may not be inherited, or which may or may not be associated with impaired DNA repair, inflammation-related autoimmunity, etc.), a specific age or age bracket, a specific ethnic group that may or may not be associated with frequent occurrence of specific type of cancer. Of course, populations may also be enlisted from databases with known omics information, and especially publically available omics information from cancer patients (e.g., TCGA, COSMIC, etc.) and proprietary databases from a large variety of individuals that may be healthy or diagnosed with a disease. Likewise, it should be appreciated that the population records may also be indexed over time for the same individual or group of individuals, which advantageously allows detection of shifts or changes in the genes and pathways associated with different types of cancers.

[0054]In further particularly preferred aspects, it is contemplated that a cancer score can be established for one or more cancer-related genes, inflammation-related genes, a DNA-repair gene, a neoepitope, and a gene not associated with a disease and that the score may be reflective of or even prognostic for various types of cancer that are at least in part due to mutations in cancer-related genes and/or pathways. For example, especially suitable cancer scores may involve scores for one or more genes associated with one or more types of cancer (e.g., BRCA1, BRCA2, P53, etc.) relative to another gene that may or may not be associated with one type of cancer (e.g., housekeeping genes, etc.). In another example, contemplated cancer scores may involve scores for one or more genes associated with one or more types of one or more types of cancer (e.g., BRCA1, BRCA2, P53, etc.) relative to an overall mutation rate (e.g., mutation rate of the genes not associated with a disease, etc.) to so better identify cancer relevant mutations over ‘background’ mutations.

[0055]Additionally, the omics data may be used to generate a general error status for an individual (or tumor within an individual), or to associate the number and/or type of alterations in cancer-related genes, inflammation-related genes, or a DNA-repair gene to identify a ‘tipping point’ for one or more gene mutations after which a general mutation rate skyrockets. For example, where a rate or number of mutations in ERCC1 and other DNA repair genes could have only minor systemic consequence, addition of further mutations to TP53 may result in a catastrophic increase in mutation rates. Thus, and viewed from a different perspective, mutations in the genes associated with DNA may be used to estimate the risk of occurrence for a DNA damage-based disease, and especially cancer and age-related diseases. In still further contemplated uses, so obtained omics information may be analyzed in one or more pathway analysis algorithms (e.g., PARADIGM) to so identify affected pathways and to so possibly adjust treatment where treatment employs DNA damaging agents. Pathway analysis algorithms may also be used to in silico modulate expression of one or more DNA repair genes, which may results in desirable or even unexpected in silico treatment outcomes, which may be translated into the clinic.

[0056]With respect to calculation, the inventors contemplate that the cancer score is typically a compound score reflecting status of a plurality of genes. For example, the cancer score can be calculated by counting any mutations (e.g., deletion, missense, nonsense, etc.) of any cancer-related genes, inflammation-related genes, and DNA-repair genes with one or more mutations as having a positive value, counting any changes in methylation or other modifications in DNA of counting any cancer-related genes, DNA-repair genes, counting any upregulation or downregulation in expression levels of RNA of any cancer-related genes, inflammation-related genes, and DNA-repair genes, counting any presence of tumor-specific, patient specific neoepitopes, counting any changes or ratios in RNA isotypes (splice variants) of counting any cancer-related genes and DNA-repair genes, and counting any changes in length of poly A tail of any cancer-related genes, inflammation-related genes, and DNA-repair genes.

[0057]The inventors further contemplate that each count may be weighed uniformly or biased, based on the significance of each count and then be assigned a value according to the weight of each count (e.g., each count corresponds to 1 point, some counts correspond to different scores such as 1 point, 3 points, 10 points, 100 points, etc.). Some mutations in some cancer related genes may be ‘leading indicators’ or triggers to activate other tumorigenesis mechanism or metastasis. Identification of such triggers may advantageously allow for early diagnosis or intervention of the cancer. Thus, for example, a mutation in a cancer-specific gene among cancer-related genes, inflammation-related genes, or DNA-repair genes may be weighed higher than other cancer-related genes or DNA-repair genes (e.g., at least 3 times, at least 5 times, at least 10 times, at least 100 times, etc.) and can be assigned to higher values accordingly. As used herein the cancer-specific gene refers any gene or mutation of the gene that is a known genetic disposition (e.g., significantly increase a susceptibility to the disease) of specific types of cancer (e.g., BRCA1 and BRCA2 for breast cancer and ovarian cancer, etc.). In another example, each gene in any cancer-related pathway or DNA-repair pathway may be differently weighed (e.g., most significant, significant, moderate, less significant, insignificant, etc.) and any mutation of a such gene that has any or no impact (e.g., adversely affect the pathway stream, etc.) on any cancer-related pathway or DNA-repair pathway may be weighed differently based on the significance of the impact. Thus, for example, gene A encoding a significant, unreplaceable protein A in a cancer pathway may be weighed heavier than another gene B encoding a redundant protein (replaceable with other proteins). Also, a nonsense mutation in gene A that results in nonfunctional protein may be weighed at least 3 times, at least 5 times, at least 10 times, at least 100 times than a silent mutation in gene A or a missense mutation which does not affect the function of protein A and can be assigned to higher values accordingly.

[0058]In some embodiments, some countings may weigh equally or differently based on the significance of each counting and then be assigned to a negative value according to the weight of each counting (e.g., each counting corresponds to −1 point, some countings correspond to different scores such as −1 point, −3 points, −10 points, −100 points, etc.). For example, upregulation of mRNA of gene C, which can compensate the loss of function of gene A, can be assigned to a negative value (e.g., −10 points) such that it can compensate the positive value of mutation of gene A (e.g., +10 points).

[0059]It is also contemplated that some countings may be differently weighed based on the degree of changes in expression level of some RNAs. For example, when the expression level of RNA “X” increases at least twice, at least 5 times, at least 10 times, at least 20 times, while other RNA expression level change is below 50% at best, then the increase of expression level of RNA “X” may be weighed at least 3 times, at least 5 times, at least 10 times, at least 100 times than other genes.

[0060]Most typically, the cancer score is compound score that is a total sum of all values assigned to all counts. In some embodiments, the cancer score can be a total sum of all values assigned to all counts (all omics data). In other embodiments, the cancer score can be a total sum of a selected number of values assigned to some counts (e.g., corresponding to specific pathways, specific types of genes, specific groups of mechanisms, etc.). Thus, the cancer score increases as more cancer-related genes or DNA-repair genes possess one or more mutations. In some embodiments, each mutation and/or change may be counted separately such that cancer scores may further increase where one or more cancer-related genes or DNA-repair genes show multiple mutations in a single gene. In other embodiments, cancer score may further increase when such multiple mutations in a single gene may further affect the function of the cancer-related genes or DNA-repair genes such that the multiple mutations drive the cells more cancer-prone, or more cancerous, or drive the cancer microenvironment more immune-resistant, and so on.

[0061]Alternatively or additionally, the cancer score can be presented as a trajectory with one or more counts as its vectors, where a few numbers of variables and/or factors dominantly govern in determination of cancer prognosis. Each of variables and/or factors can be presented as a vector, whose amplitude is corresponding to the point of each weighted counting, and the addition of those vectors provides a trajectory indicating the prognosis of the disease. Viewed form a different perspective, it should be appreciated that multiple analyses over time can be prepared for the same patient, and that changes over time (e.g., with or without treatment) may be assigned specific values that will yet again generate a time-dependent score. Such scores or changes over time may be classified and serve as leading indicator for treatment outcome, drug response, etc.

[0062]Additionally, it is also contemplated that the cancer score can be calculated with health information other than cf/ct nucleic acid data obtained from the patient's blood. For example, the health information may include expression levels/concentrations of several types of cytokines (e.g., IL-2, TNF-α, etc.) related to tumorigenesis/inflammation/immune response against the tumor, hormone levels (e.g., estrogen, progesterone, growth hormone, etc.), blood sugar level, alanine transaminase level (for liver function), creatine level (for kidney function), blood pressure, types and quantity of tumor cell-secreted proteins (e.g., soluble ligands of immune cell receptor, etc.) or foreign antigenic proteins (e.g., for virus or bacterial infection, etc.).

[0063]The inventors contemplated that the so obtained cancer score can be used to provide a diagnosis of cancer or risk of having or developing a cancer. In some embodiments, the calculated cancer score of a patient can be compared with an average cancer score of healthy individuals to determine the difference between two scores. Preferably, when the difference between two scores is above a threshold value, the patient may be diagnosed to have a tumor, or has a high risk to have a tumor. In other embodiments, the calculated cancer score of a patient can be compared with a predetermined threshold score. The predetermined threshold score can be a predetermined score, which may vary depending on patient's ethnicity, age, gender, or other health status. In other embodiments, the predetermined threshold score can a dynamic score that can be changed based on a previous cancer score and a diagnosis or treatment performed to the patient.

[0064]The inventors also contemplate that the so obtained cancer score can be used to provide a prognosis of the cancer. For example, the cancer scores can be calculated based on omics data obtained in month 1, month 3, month 6, and month 12 after the patient got diagnosed with a first stage of lung cancer, and each cancer score can be compared with a predetermined threshold score corresponding to the month 1, 3, 6, and 12. The cancer scores are about 120% of the threshold score in month 1 and 3, and the cancer score is about 180% in month 6, and 230% of the threshold score month 12. Such progress indicates that the prognosis of the lung cancer of the patient is not optimistic if the progress is not intervened. In another example, the cancer score can be calculated by highly weighing the presence of neoepitopes that are tumor-specific and patient-specific. In this example, the cancer scores can be calculated based on omics data obtained in month 1, month 3, month 6, and month 12 after the patient got diagnosed with a first stage of lung cancer, and each cancer score is calculated by highly weighing the presence/appearance of new epitope that is tumor/tissue specific. The cancer scores are about 120% of the threshold score in month 1 and 3, and the cancer score is about 140% in month 6, and 230% of the threshold score month 12. Such progress indicates a possible metastasis of the tumor to another organ (releasing different type of neoepitope) or development of different type of tumor in the same organ (releasing different type of neoepitope).

[0065]In a further example, the cancer scores can provide an indicator for treatment options. The treatment option may be a prophylactic treatment where the compound score is below the threshold value, indicating that the patient is unlikely to have a tumor for now or at least has low risk of developing a tumor. When the cancer score is above the threshold value and a majority portion of the cancer score highly weighted was overexpression of a cancer-related gene A (e.g., over a threshold such as at least 10%, at least 20%, at least 30%, at least 50%, etc.), then the cancer score can be used to provide the treatment option that may use a drug inhibiting the activity of cancer-related gene A (e.g., a blocker of protein A, etc.). Similarly, when the cancer score is above the threshold value and a majority portion of the cancer score highly weighted was overexpression of a gene encoding a receptor of an immune cell or a ligand of the receptor, then the cancer score can be used to provide the immunotherapy using the receptor or ligand of the immune cells. Also, when the cancer score is above the threshold value and a majority portion of the cancer score highly weighted was overexpression of a specific neoepitope, then the cancer score can be used to provide the immunotherapy using the neoepitope as a bait or a surgery/a radiation therapy to physically remove local tumors. Also such cancer scores may be an indicative of likelihood of success for the treatment option. However, if the portion of the cancer score highly weighted was overexpression of a cancer-related gene A is below the threshold, then the treatment option using a drug inhibiting the activity of cancer-related gene A may be predicted less effective.

[0066]Consequently, the patient can be treated with at least one of the treatment options based on the patient's cancer (compound) score. For example, above the threshold value and a majority portion of the cancer score highly weighted was overexpression of a specific neoepitope, the treatment option can be selected to include a recombinant virus (or yeast or bacteria) comprising a nucleic acid encoding the specific neoepitope. Then, the recombinant virus can be administered to the patient in a dose and schedule effective to treat the tumor and/or effective to reduce the cancer score of the patient for at least 10%, at least 20%, at least 30%, at least in 2 weeks, at least in 4 weeks, at least in 8 weeks, at least in 12 weeks after the administration or a series of administrations.

[0067]It is also contemplated that the patient's cancer score can be compared with one or more other patients having same type of cancer and having a treatment history to provide a treatment option and predicted outcome. For example, where other patients' history indicates that the drug treatment is effective only when the cancer score is below 200 (as absolute score), or less than 180% of the healthy individual's score, and the patient's cancer score has been increasing from 140 to 160 for the last 2 weeks, a recommendation to proceed with drug treatment no later than 2 weeks can be provided based on the other patients' history and cancer scores.

[0068]The calculated cancer score can also be an indicator of an effectiveness of a cancer treatment, especially when the omics data includes information of at least one or more genes encoding a target/indicator of the cancer treatment. For example, cancer scores can be calculated based on omics data obtained before the cancer treatment, 7 days after, 2 weeks, 1 month, and 6 months of the cancer treatment. The cancer score of 7 days after the treatment is 80% of the cancer score before the treatment, and the cancer score of 2 weeks and 1 month after the treatment is 50% of the cancer score before the treatment, and the cancer score of 6 months after the treatment is 150% of the cancer score before the treatment. Such progress indicates that the treatment was effective at least for a short term (e.g., up to 1 month), yet the effectiveness is decreased over time and may not effective at all in 6 months after the treatment. In some embodiments, the cancer scores before and after treatment can be compared with a predetermined threshold value to determine the effectiveness of the treatment. For example, if the cancer score is 200 before the treatment and 130 after the treatment where the threshold cancer score is 100, then the treatment can be determined “effective” as the cancer score drops below the threshold after the treatment. However, if the cancer score is 200 before the treatment and 160 after the treatment where the threshold cancer score is 150, then the treatment can be determined “not effective” as the cancer score stays above the threshold after the treatment even though the absolute value of the cancer score is decreased. Consequently, the inventors further contemplate that the patient continues with administering the treatment option (e.g., immune therapy, etc.) when the treatment can be determined “effective”, when the cancer score after the treatment is lower than the predetermined threshold, when the cancer score after the treatment is at most 5%, at most 10% higher than the predetermined threshold, or when the cancer score after the treatment is at least 5%, at least 10%, at least 15% lower than the predetermined threshold. s

[0069]The inventors also contemplate that the effectives of some cancer treatments can be determined by analyzing omics data including foreign DNA/RNA originated from a carrier of the immune therapy (e.g., virus, bacteria, yeast, etc.). For example, where the virus is a carrier to deliver a recombinant nucleic acid encoding recombinant killer activation receptor (KAR), the level of cell free DNA/RNA of recombinant KAR in the patient blood can be an indicator of an effectiveness of infection of the virus.

[0070]It should be apparent to those skilled in the art that many more modifications besides those already described are possible without departing from the inventive concepts herein. The inventive subject matter, therefore, is not to be restricted except in the scope of the appended claims. Moreover, in interpreting both the specification and the claims, all terms should be interpreted in the broadest possible manner consistent with the context. In particular, the terms “comprises” and “comprising” should be interpreted as referring to elements, components, or steps in a non-exclusive manner, indicating that the referenced elements, components, or steps may be present, or utilized, or combined with other elements, components, or steps that are not expressly referenced. As used in the description herein and throughout the claims that follow, the meaning of “a,” “an,” and “the” includes plural reference unless the context clearly dictates otherwise. Also, as used in the description herein, the meaning of “in” includes “in” and “on” unless the context clearly dictates otherwise. Where the specification claims refers to at least one of something selected from the group consisting of A, B, C . . . and N, the text should be interpreted as requiring only one element from the group, not A plus N, or B plus N, etc.

Claims

What is claimed is:

1. A method of evaluating an effectiveness of a treatment for a cancer patient, comprising:

obtaining blood from a patient having a cancer;

obtaining from the blood omics data of the cancer patient before and after the treatment for a plurality of cancer-related genes, wherein the omics data comprise at least one of DNA sequence data, RNA sequence data, and RNA expression level;

analyzing the omics data to generate first and second cancer gene scores, wherein the first and cancer gene scores correspond to the omics data before and after the treatment, respectively; and

providing the effectiveness of the treatment based on a comparison of the first and second cancer gene scores.

2. The method of claim 1, wherein the plurality of cancer-related genes comprises at least one of a cancer-related gene, a cancer-specific gene, a DNA-repair gene, a neoepitope, and a gene not associated with a disease.

3. The method of claim 2, wherein the neoepitope is tumor specific and patient specific.

4. The method of claim 1, wherein the DNA sequence data are selected from the group consisting of mutation data, copy number data duplication, loss of heterozygosity data, and epigenetic status.

5. The method of claim 1, wherein the RNA sequence data are selected from the group consisting of mRNA sequence data and splice variant data.

6. The method of claim 1, wherein the RNA expression level data are selected from the group consisting of a quantity of RNA transcript and a quantity of a small noncoding RNA.

7. The method of claim 1, wherein DNA sequence data are obtained from circulating free DNA.

8. The method of claim 1, wherein the RNA sequence data are obtained from the group consisting of circulating tumor RNA and circulating free RNA.

9. The method of claim 4, wherein the plurality of cancer-related genes includes a cancer-specific gene, and the score is calculated based on a presence or an absence of a mutation in the cancer-specific gene.

10. The method of claim 9, wherein the presence of the mutation in the cancer-specific gene weighs more than the presence of the mutation in the cancer-related genes other than the cancer-specific gene.

11. The method of claim 5, wherein the score is calculated based on a type of a splice variant of the cancer gene or a ratio between a plurality of splice variants of the cancer gene.

12. The method of claim 1, wherein the treatment is a drug, and at least one of the plurality of cancer gene is a predicted target of the drug.

13. The method of claim 1, wherein the treatment is an immune therapy, and at least one of the plurality of cancer gene is a receptor of an immune cell or a ligand of the receptor.

14. The method of claim 1, wherein the treatment is a surgery or a radiation therapy, and at least one of the plurality of cancer gene is a neoepitope that is tumor-specific and patient-specific.

15. The method of claim 1, wherein the effectiveness of the treatment is determined by comparing the cancer gene score after the treatment with a predetermined threshold value.

16. The method of claim 1, wherein the effectiveness of the treatment is determined by a difference between the cancer gene score before and after the treatment.

17. The method of claim 16, wherein the treatment is determined effective when the difference is higher than a predetermined threshold value.