KR20230150127A - Genetic polymorphisms associated with myocardial infarction and uses thereof - Google Patents

Abstract

Disclosed herein are genetic polymorphisms associated with myocardial infarction and their uses. More specifically, a composition for predicting or diagnosing myocardial infarction comprising an agent for detecting a polynucleotide containing a single nucleotide polymorphism associated with myocardial infarction or a polynucleotide with a sequence complementary thereto, myocardial infarction comprising an agent for detecting the polynucleotide A kit for predicting or diagnosing infarction, and a method for providing information for predicting or diagnosing myocardial infarction including the step of detecting the polymorphic site are disclosed.

Description

Genetic polymorphisms associated with myocardial infarction and their uses {GENETIC POLYMORPHISMS ASSOCIATED WITH MYOCARDIAL INFARCTION AND USES THEREOF}

Disclosed herein are novel genetic polymorphisms associated with myocardial infarction and their uses.

Acute myocardial infarction (AMI) is one of the leading causes of death, and more than 1 million people worldwide die from acute myocardial infarction every year. Acute myocardial infarction is influenced by both genetic and environmental risk factors. The majority of acute myocardial infarctions occur in people over 65 years of age, but early-on-set acute myocardial infarction is rare (prevalence 1-5%), and genetic risk factors are more influential in early-on-set acute myocardial infarction. (Document Consortium MIG. Genome-wide association of early-onset myocardial infarction with single nucleotide polymorphisms and copy number variants. Nature genetics. 2009;41:334. etc.)

Meanwhile, in the biotechnology and medical industries, discovering genetic markers associated with diseases is important for predicting diseases and identifying congenital causes of diseases. In order to discover disease-related genetic markers, it is necessary to compare genomic data between diseased and healthy control groups.

Genome-wide association study (GWAS) is a representative method for comparing genomic data between diseased and control groups. GWAS can find disease-related genetic markers using statistical methods such as logistic regression on genetic mutations and the frequency of genetic mutations in diseased patients and control groups.

The present inventors performed Whole-genome Sequencing (WGS)-based GWAS analysis to find new genetic markers, and as a result, single nucleotide polymorphisms (Single Nucleotide polymorphisms) that can predict the probability and genetic susceptibility to myocardial infarction, especially early-onset myocardial infarction, were identified. Polymorphism (SNP) was discovered to lead to the present invention.

Therefore, in one aspect, the present invention seeks to provide specific SNPs associated with myocardial infarction, particularly early-onset myocardial infarction.

In another aspect, the present invention seeks to provide a polynucleotide containing the above SNP or a polynucleotide of a complementary sequence thereof, or a polynucleotide hybridizing therewith, as a genetic marker associated with myocardial infarction, especially early-onset myocardial infarction.

In another aspect, the present invention seeks to provide a composition for predicting or diagnosing myocardial infarction, including an agent for detecting the polynucleotide or a polynucleotide of a complementary sequence thereof.

In another aspect, the present invention seeks to provide a kit for predicting or diagnosing myocardial infarction, including an agent for detecting the polynucleotide or a polynucleotide of a complementary sequence thereof.

In another aspect, the present invention seeks to provide a method of providing information for predicting or diagnosing myocardial infarction or a method of calculating the risk of myocardial infarction, including the step of detecting the SNP.

In one aspect, the present invention provides rs1277393322, rs10810978, rs1351282285, rs1560389462, rs10235820, rs2323404, rs7641082, rs8009869, rs1405402, rs1918101, rs7 641013, rs10232190, rs200715251, rs1918100, rs9855437, rs941068, rs6770247, rs1526719, rs80334730, rs77800378, rs12487132, rs9873508, rs1526708, rs1958821, rs591012, rs1526709, rs200514416, rs111432322, rs34330766, rs7638747, rs10589173, rs12639020, rs1263 9023, rs239576, rs7759915, rs372341820, rs78631167, rs527249040, rs184610791, rs1614576, rs1657538, rs1657545, rs240224, rs7232479, rs1 3099537, rs152042, rs131570, rs7191762, rs4584426, rs152041, rs11649332, rs147169123, rs55819522, rs6573071, rs12447763, rs2520017, rs2520019, rs1164211 6, rs7196602, rs2334246, rs194817, rs168974, rs183172, rs2152884, rs141073026, rs200261514, rs5072, rs109592, rs56265975, rs12438548, rs 199830494, rs113612782, rs187748, rs174217, rs2520009, rs194797, rs117684941, rs4901620, rs12921822, rs194800, rs10852254, rs194815, rs194813, rs A polynucleotide containing one or more polymorphisms selected from the group consisting of 174219 and rs9357455, or a polynucleotide with a sequence complementary thereto Provided is a composition for predicting or diagnosing myocardial infarction containing an agent that detects.

In another aspect, the present invention provides a kit for predicting or diagnosing myocardial infarction comprising the above-described detection agent.

In another aspect, the present invention provides rs1277393322, rs10810978, rs1351282285, rs1560389462, rs10235820, rs2323404, rs7641082, rs8009869, rs1405402, rs1918101, rs from a sample. 7641013, rs10232190, rs200715251, rs1918100, rs9855437, rs941068, rs6770247, rs1526719, rs80334730, rs77800378, rs12487132 , rs9873508, rs1526708, rs1958821, rs591012, rs1526709, rs200514416, rs111432322, rs34330766, rs7638747, rs10589173, rs12639020, rs12 639023, rs239576, rs7759915, rs372341820, rs78631167, rs527249040, rs184610791, rs1614576, rs1657538, rs1657545, rs240224, rs7232479, rs13099537, rs152042 , rs131570, rs7191762, rs4584426, rs152041, rs11649332, rs147169123, rs55819522, rs6573071, rs12447763, rs2520017, rs2520019, rs11642 116, rs7196602, rs2334246, rs194817, rs168974, rs183172, rs2152884, rs141073026, rs200261514, rs5072, rs109592, rs56265975, rs12438548, rs199830494 , rs113612782, rs187748, rs174217, rs2520009, rs194797, rs117684941, rs4901620, rs12921822, rs194800, rs10852254, rs194815, rs194813, Prediction of myocardial infarction, comprising the step of detecting one or more polymorphic sites selected from the group consisting of rs174219 and rs9357455. Alternatively, it provides a method of providing information for diagnosis or a method of calculating the risk of myocardial infarction.

SNPs according to exemplary embodiments of the present invention can be used as genetic markers associated with myocardial infarction to effectively predict or calculate the risk of myocardial infarction or enable early diagnosis of myocardial infarction.

Figure 1 shows myocardial infarction-related characteristics of subjects according to an embodiment of the present invention.
Figure 2 is a Manhattan plot of acute myocardial infarction-related loci through GWAS according to an embodiment of the present invention.
Figure 3 is a table showing new loci for acute myocardial infarction according to an embodiment of the present invention.
Figure 4 shows eQTL for a myocardial infarction-related locus according to an embodiment of the present invention.

The terms used in this specification are general terms that are currently widely used as much as possible while considering the function in the present invention, but this may vary depending on the intention of a technician working in the field, precedents, or the emergence of new technology. In addition, in certain cases, there are terms arbitrarily selected by the applicant, and in this case, the meaning will be described in detail in the description of the relevant invention. Therefore, the terms used in this specification should be defined based on the meaning of the term and the overall content of the present invention, rather than simply the name of the term.

Unless otherwise defined, all terms used herein, including technical or scientific terms, have the same meaning as generally understood by a person of ordinary skill in the technical field to which the present invention pertains. Generally understood terms should be interpreted as having the same meaning as the meaning they have in the context of the related technology, and unless clearly defined in the present invention, they should not be interpreted in an idealized or excessively formal sense.

Numerical ranges include the numerical values defined herein. Every maximum numerical limit given throughout this specification includes all lower numerical limits as if the lower numerical limit were explicitly written out. Every minimum numerical limit given throughout this specification includes every higher numerical limit as if such higher numerical limit was clearly written. All numerical limits given throughout this specification will include all better numerical ranges within the broader numerical range, as if the narrower numerical limits were clearly written.

As used herein, the words “comprising,” “having,” and “comprising” are inclusive or open-ended and do not exclude additional unstated elements or method steps. As used herein, the term “or combination thereof” refers to all permutations and combinations of the items listed preceding the term. For example, "A, B, C, or any combination thereof" means A, B, C, AB, AC, BC, or ABC, and, if the order is important in a particular context, BA, CA, CB, CBA, BCA. , it is intended to include at least one of ACB, BAC or CAB. Along with this example, combinations containing repetitions of one or more items or terms may be included, such as BB, AAA, MB, BBC, AAABCCCC, CBBAAA, CABABB, etc. Those skilled in the art will understand that there is typically no limit to the number of items or terms in any combination, unless otherwise apparent from the context.

In one aspect of the present invention, a polymorphism related to a specific function may be related to other functions in addition to being related to the specific function, and is not excluded from being related to two or more functions. For example, at least a polymorphism related to thrombosis may mean a polymorphism related not only to thrombosis but also to other functions.

In one aspect of the present invention, “genetic marker”, “biomarker” or “marker” refers to a substance that can diagnose myocardial infarction or predict or calculate the risk of myocardial infarction, and is associated with a higher risk of myocardial infarction compared to the normal group. It includes organic biomolecules such as polypeptides or nucleic acids, lipids, glycolipids, glycoproteins, and sugars (monosaccharides, disaccharides, oligosaccharides, etc.) that show an increase or decrease depending on the condition. Genetic markers provided in exemplary embodiments of the present invention are clearly listed in Tables 1 to 12, with 85 genetic variants. The markers themselves may indicate SNPs, cryptic splicing and other genetic defects.

In one aspect of the invention, “complementary” means sufficiently complementary to selectively hybridize to a target nucleic acid sequence under predetermined annealing or hybridization conditions, and encompasses substantially complementary and/or fully complementary. It can be. Accordingly, “complementary” sequences may include not only completely identical sequences but also sequences that partially mismatch the sequence to be compared to the extent that they can selectively hybridize to a specific sequence.

In one aspect of the present invention, “myocardial infarction” may particularly include acute myocardial infarction, early-onset myocardial infarction, or early-onset acute myocardial infarction.

In one aspect of the invention, “early onset” means onset at age 50 or younger for men and age 60 or younger for women.

In one aspect of the present invention, "myocardial infarction prediction" refers to predicting or diagnosing whether a subject is likely to develop myocardial infarction, whether the likelihood of developing myocardial infarction is relatively high, and what the causative factor of myocardial infarction is. It may mean that it includes something.

In one aspect of the present invention, “myocardial infarction diagnosis” means confirming the presence or characteristics of a pathological condition in a subject, and for the purpose of one aspect of the present invention, diagnosis means confirming whether myocardial infarction has occurred. It can mean.

In one aspect of the present invention, "calculating the risk of myocardial infarction" refers to assessing whether the likelihood of developing myocardial infarction in a subject is relatively high or low, increases or decreases compared to the case where a genetic marker is present or not present. It may mean including doing.

In one aspect of the present invention, the types and numbers of the genetic markers may be used in various combinations to suit various purposes such as predicting, diagnosing, and calculating risk of myocardial infarction described above.

The composition, kit or method according to one aspect of the present invention can be used to delay the onset of myocardial infarction or prevent it from occurring through special and appropriate management for subjects at high risk of developing myocardial infarction.

Hereinafter, exemplary embodiments of the present invention will be described in detail. However, it is obvious that the present invention is not limited to the following embodiments.

In one aspect, exemplary embodiments of the invention include rs1277393322, rs10810978, rs1351282285, rs1560389462, rs10235820, rs2323404, rs7641082, rs8009869, rs1405402, rs191810. 1, rs7641013, rs10232190, rs200715251, rs1918100, rs9855437, rs941068, rs6770247, rs1526719, rs80334730 , rs77800378, rs12487132, rs9873508, rs1526708, rs1958821, rs591012, rs1526709, rs200514416, rs111432322, rs34330766, rs7638747, rs10 589173, rs12639020, rs12639023, rs239576, rs7759915, rs372341820, rs78631167, rs527249040, rs184610791, rs1614576, rs1657538, rs165754 5, rs240224, rs7232479 , rs13099537, rs152042, rs131570, rs7191762, rs4584426, rs152041, rs11649332, rs147169123, rs55819522, rs6573071, rs12447763, rs25200 17, rs2520019, rs11642116, rs7196602, rs2334246, rs194817, rs168974, rs183172, rs2152884, rs141073026, rs200261514, rs5072, rs109592, rs 56265975 , rs12438548, rs199830494, rs113612782, rs187748, rs174217, rs2520009, rs194797, rs117684941, rs4901620, rs12921822, rs194800, rs1085 A polynucleotide containing one or more polymorphisms selected from the group consisting of 2254, rs194815, rs194813, rs174219 and rs9357455, or complementary thereto A composition for predicting or diagnosing myocardial infarction comprising an agent that detects a polynucleotide of a suitable sequence is provided.

In one embodiment, rs1277393322 may predict or diagnose myocardial infarction when the 28772995th base of human chromosome 20 is A.

In one embodiment, rs10810978 may predict or diagnose myocardial infarction when the 18523845th base of human chromosome 9 is C.

In one embodiment, rs1351282285 may predict or diagnose myocardial infarction when the 164704630th base of human chromosome 3 is T.

In one embodiment, rs1560389462 may predict or diagnose myocardial infarction when the 195788126th base of human chromosome 3 is G.

In one embodiment, rs10235820 may predict or diagnose myocardial infarction when the 32082944th base of human chromosome 7 is A.

In one embodiment, rs2323404 may predict or diagnose myocardial infarction when the 73926364th base of human chromosome 3 is A.

In one embodiment, rs7641082 may predict or diagnose myocardial infarction when the 73923420th base of human chromosome 3 is T.

In one embodiment, rs8009869 may predict or diagnose myocardial infarction when the 55900262nd base of human chromosome 14 is G.

In one embodiment, rs1405402 may predict or diagnose myocardial infarction when the 73921969th base of human chromosome 3 is G.

In one embodiment, rs1918101 may predict or diagnose myocardial infarction when the 73927087th base of human chromosome 3 is G.

In one embodiment, rs7641013 may predict or diagnose myocardial infarction when the 73923383rd base of human chromosome 3 is T.

In one embodiment, rs10232190 may predict or diagnose myocardial infarction when the 152231944th base of human chromosome 7 is A.

In one embodiment, rs200715251 may predict or diagnose myocardial infarction when the 30175826th base of human chromosome 15 is G.

In one embodiment, rs1918100 may predict or diagnose myocardial infarction when the 73927219th base of human chromosome 3 is T.

In one embodiment, rs9855437 may predict or diagnose myocardial infarction when the 73925188th base of human chromosome 3 is A.

In one embodiment, rs941068 may predict or diagnose myocardial infarction when the 73925641st base of human chromosome 3 is C.

In one embodiment, rs6770247 may predict or diagnose myocardial infarction when the 73927363rd base of human chromosome 3 is G.

In one embodiment, rs1526719 may predict or diagnose myocardial infarction when the 73927320th base of human chromosome 3 is G.

In one embodiment, rs80334730 may predict or diagnose myocardial infarction when the 55906845th base of human chromosome 14 is C.

In one embodiment, rs77800378 may predict or diagnose myocardial infarction when the 55907084th base of human chromosome 14 is A.

In one embodiment, rs12487132 may predict or diagnose myocardial infarction when the 73919134th base of human chromosome 3 is A.

In one embodiment, rs9873508 may predict or diagnose myocardial infarction when the 73925782nd base of human chromosome 3 is G.

In one embodiment, rs1526708 may predict or diagnose myocardial infarction when the 73918804th base of human chromosome 3 is G.

In one embodiment, rs1958821 may predict or diagnose myocardial infarction when the 55908821st base of human chromosome 14 is C.

In one embodiment, rs591012 may predict or diagnose myocardial infarction when the 80038900th base of human chromosome 6 is G.

In one embodiment, rs1526709 may predict or diagnose myocardial infarction when the 73918900th base of human chromosome 3 is C.

In one embodiment, rs200514416 may predict or diagnose myocardial infarction when the 87414203rd base of human chromosome 9 is C.

In one embodiment, rs111432322 may predict or diagnose myocardial infarction when the 55905697th base of human chromosome 14 is T.

In one embodiment, rs34330766 may predict or diagnose myocardial infarction when the 73924589th base of human chromosome 3 is A.

In one embodiment, rs7638747 may predict or diagnose myocardial infarction when the 73923365th base of human chromosome 3 is A.

In one embodiment, rs10589173 may predict or diagnose myocardial infarction when the 55905174th base of human chromosome 14 is A.

In one embodiment, rs12639020 may predict or diagnose myocardial infarction when the 73919588th base of human chromosome 3 is C.

In one embodiment, rs12639023 may predict or diagnose myocardial infarction when the 73919636th base of human chromosome 3 is C.

In one embodiment, rs239576 may predict or diagnose myocardial infarction when the 80021249th base of human chromosome 6 is G.

In one embodiment, rs7759915 may predict or diagnose myocardial infarction when the 80062270th base of human chromosome 6 is T.

In one embodiment, rs372341820 may predict or diagnose myocardial infarction when the 29655837th base of human chromosome 16 is A.

In one embodiment, rs78631167 may predict or diagnose myocardial infarction when the 43676115th base of human chromosome 19 is C.

In one embodiment, rs527249040 may predict or diagnose myocardial infarction when the 1029328th base of human chromosome 19 is C.

In one embodiment, rs184610791 may predict or diagnose myocardial infarction when the 39788017th base of the human X chromosome is G.

In one embodiment, rs1614576 may predict or diagnose myocardial infarction when the 23747804th base of human chromosome 16 is G.

In one embodiment, rs1657538 may predict or diagnose myocardial infarction when the 23747877th base of human chromosome 16 is A.

In one embodiment, rs1657545 may predict or diagnose myocardial infarction when the 23748316th base of human chromosome 16 is G.

In one embodiment, rs240224 may predict or diagnose myocardial infarction when the 80007571st base of human chromosome 6 is G.

In one embodiment, rs7232479 may predict or diagnose myocardial infarction when the 15377667th base of human chromosome 18 is A.

In one embodiment, rs13099537 may predict or diagnose myocardial infarction when the 73923060th base of human chromosome 3 is T.

In one embodiment, rs152042 may predict or diagnose myocardial infarction when the 23754252nd base of human chromosome 16 is G.

In one embodiment, rs131570 may predict or diagnose myocardial infarction when the 16400343rd base of human chromosome 22 is C.

In one embodiment, rs7191762 may predict or diagnose myocardial infarction when the 23741456th base of human chromosome 16 is A.

In one embodiment, rs4584426 may predict or diagnose myocardial infarction when the 247921552nd base of human chromosome 1 is G.

In one embodiment, rs152041 may predict or diagnose myocardial infarction when the 23754034th base of human chromosome 16 is C.

In one embodiment, rs11649332 may predict or diagnose myocardial infarction when the 23748912th base of human chromosome 16 is T.

In one embodiment, rs147169123 may predict or diagnose myocardial infarction when the 25189022nd base of human chromosome 9 is A.

In one embodiment, rs55819522 may predict or diagnose myocardial infarction when the 23771655th base of human chromosome 16 is T.

In one embodiment, rs6573071 may predict or diagnose myocardial infarction when the 55904081st base of human chromosome 14 is A.

In one embodiment, rs12447763 may predict or diagnose myocardial infarction when the 23742273rd base of human chromosome 16 is T.

In one embodiment, rs2520017 may predict or diagnose myocardial infarction when the 23784944th base of human chromosome 16 is A.

In one embodiment, rs2520019 may predict or diagnose myocardial infarction when the 23785567th base of human chromosome 16 is C.

In one embodiment, rs11642116 may predict or diagnose myocardial infarction when the 23786091st base of human chromosome 16 is C.

In one embodiment, rs7196602 may predict or diagnose myocardial infarction when the 23786294th base of human chromosome 16 is T.

In one embodiment, rs2334246 may predict or diagnose myocardial infarction when the 23787611th base of human chromosome 16 is T.

In one embodiment, rs194817 may predict or diagnose myocardial infarction when the 23788500th base of human chromosome 16 is A.

In one embodiment, rs168974 may predict or diagnose myocardial infarction when the 23789042nd base of human chromosome 16 is A.

In one embodiment, rs183172 may predict or diagnose myocardial infarction when the 23789509th base of human chromosome 16 is C.

In one embodiment, rs2152884 may predict or diagnose myocardial infarction when the 237214855th base of human chromosome 1 is A.

In one embodiment, rs141073026 may predict or diagnose myocardial infarction when the 61717206th base of human chromosome 1 is C.

In one embodiment, rs200261514 may predict or diagnose myocardial infarction when the 73222956th base of human chromosome 12 is GTAAT.

In one embodiment, rs5072 may predict or diagnose myocardial infarction when the 116836867th base of human chromosome 11 is A.

In one embodiment, rs109592 may predict or diagnose myocardial infarction when the 23757389th base of human chromosome 16 is T.

In one embodiment, rs56265975 may predict or diagnose myocardial infarction when the 23759927th base of human chromosome 16 is G.

In one embodiment, rs12438548 may predict or diagnose myocardial infarction when the 36119067th base of human chromosome 15 is G.

In one embodiment, rs199830494 may predict or diagnose myocardial infarction when the 32154607th base of human chromosome 9 is G.

In one embodiment, rs113612782 may predict or diagnose myocardial infarction when the 23761303rd base of human chromosome 16 is A.

In one embodiment, rs187748 may predict or diagnose myocardial infarction when the 23767186th base of human chromosome 16 is A.

In one embodiment, rs174217 may predict or diagnose myocardial infarction when the 23768995th base of human chromosome 16 is G.

In one embodiment, rs2520009 may predict or diagnose myocardial infarction when the 23769092nd base of human chromosome 16 is T.

In one embodiment, rs194797 may predict or diagnose myocardial infarction when the 23769518th base of human chromosome 16 is C.

In one embodiment, rs117684941 may predict or diagnose myocardial infarction when the 18556791st base of human chromosome 12 is C.

In one embodiment, rs4901620 may predict or diagnose myocardial infarction when the 55901317th base of human chromosome 14 is A.

In one embodiment, rs12921822 may predict or diagnose myocardial infarction when the 7002773rd base of human chromosome 16 is C.

In one embodiment, rs194800 may predict or diagnose myocardial infarction when the 23763247th base of human chromosome 16 is C.

In one embodiment, rs10852254 may predict or diagnose myocardial infarction when the 23790378th base of human chromosome 16 is C.

In one embodiment, rs194815 may predict or diagnose myocardial infarction when the 23790834th base of human chromosome 16 is G.

In one embodiment, rs194813 may predict or diagnose myocardial infarction when the 23791390th base of human chromosome 16 is C.

In one embodiment, rs174219 may predict or diagnose myocardial infarction when the 23791599th base of human chromosome 16 is C.

In one embodiment, rs9357455 may predict or diagnose myocardial infarction when the 12693654th base of human chromosome 6 is C.

The composition according to an aspect of the present invention may be applied to a sample of a subject, and the sample refers to any sample obtained from an individual in which the expression of a marker according to an aspect of the present invention can be detected, specifically, for example, In addition to blood, it may be one or more selected from various tissues derived from the human body, saliva, biopsy, liquid culture, feces, and urine, but is not limited thereto, and is not limited to one or more of those commonly used in the technical field of the present invention. It can be prepared by processing in this way.

As a non-limiting example, the sample may include one or more selected from tissues, cells, body fluids, feces, urine, plasma, serum, whole blood, cells isolated from blood, and cell-free polynucleotides.

In another aspect, exemplary embodiments of the present invention provide a kit for predicting or diagnosing myocardial infarction comprising an agent or composition for detecting the polynucleotide or a polynucleotide of a sequence complementary thereto.

In one embodiment, the agent may include a primer pair or probe that specifically binds to the polynucleotide or a polynucleotide of a sequence complementary thereto.

In one aspect of the present invention, "primer" refers to a base of a sequence that can bind complementary to the end of a specific region of a gene used to amplify a specific region corresponding to the target region of a gene using PCR, etc. It may mean a polynucleotide (including oligonucleotide) or a variant thereof. The primer is not required to be completely complementary to the end of a specific region, and can be used as long as it is complementary enough to hybridize to the end to form a double chain structure.

In one embodiment, the primers are used for template-directed DNA synthesis under appropriate conditions (e.g., four different nucleoside triphosphates and a polymerizer such as DNA, RNA polymerase, or reverse transcriptase) in an appropriate buffer and at an appropriate temperature. It may refer to a single-stranded oligonucleotide that can act as a starting point. It consists of a pair of forward and reverse primers, and usually has a length of 7 to 50 nucleic acids, more preferably 10 to 30 nucleic acids. Short primer molecules generally require lower temperatures to form stable hybrids with the template. As mentioned above, the primer sequence need not be completely complementary to the template, but should be sufficiently complementary to hybridize to the template. The primer hybridizes to the target DNA containing the polymorphic site, and the primer initiates amplification of the allelic form showing complete homology. This primer can be used in pair with a second primer that hybridizes to the opposite side.

Meanwhile, in one aspect of the present invention, “probe” refers to a polynucleotide (including oligonucleotides), a variant thereof, or a polynucleotide having a base sequence capable of complementary binding to the target site of a gene. This may mean including a labeling substance bound thereto.

If necessary, the primer nucleic acid sequence according to one embodiment of the present invention may include a label detectable directly or indirectly by spectroscopic, photochemical, biochemical, immunochemical or chemical means. Examples of labels include enzymes (e.g., horseradish peroxidase, alkaline phosphatase), radioisotopes (e.g., 33P), fluorescent molecules, chemical groups (e.g., biotin), etc. there is.

In one embodiment, the probe refers to a nucleic acid fragment such as RNA or DNA that is as short as a few bases or as long as several hundreds of bases, capable of forming sequence-specific binding to the complementary strand of a nucleic acid, and is labeled, so that it can bind to a specific gene. You can check its presence or absence. The probe may be, for example, in the form of an oligonucleotide probe, a single stranded DNA probe, a double stranded DNA probe, an RNA probe, etc.

In one embodiment, the agent may be an agent that detects the polypeptide encoded by the polynucleotide, for example, an antibody.

In one embodiment, the antibody may be one or more selected from the group consisting of polyclonal antibodies, monoclonal antibodies, recombinant antibodies, and combinations thereof. Specifically, the antibody is a complete form having two full-length light chains and two full-length heavy chains, as well as functional fragments of the antibody molecule, such as Fab, F(ab'), F(ab')2. and Fv. Antibodies can be easily produced using techniques well known in the field to which the present invention pertains, and antibodies that have been manufactured and sold commercially can be used.

In one embodiment, the kit may be a kit for RT-PCR, competitive RT-PCR, real-time RT-PCR, RNase protection assay, Northern blotting, DNA microarray chip, or sequencing, but is not limited thereto. In addition, the kit containing an agent for detecting the polypeptide encoded by the polynucleotide may be, for example, ELISA, radioimmunoassay, tissue immunostaining, protein chip kit, etc., but is not limited thereto. Additionally, the kit may be composed of one or more different component compositions, solutions, or devices suitable for the analysis method.

For example, a kit for RT-PCR contains, in addition to each primer pair specific for a marker gene, test tubes or other suitable containers, reaction buffer (pH and magnesium concentration vary), deoxynucleotides (dNTPs), Taq-polymer It may include enzymes such as enzymes and reverse transcriptase, DNAse, RNAse inhibitors, DEPC-water, sterilized water, etc. It may also include a primer pair specific for the gene used as a quantitative control.

Additionally, for example, a kit for a DNA microarray chip includes a substrate to which a cDNA corresponding to a gene or a fragment thereof is attached as a probe, and the substrate may include a cDNA corresponding to a quantitative control gene or a fragment thereof.

In one embodiment, in the agent, composition, or kit, the myocardial infarction may be an acute myocardial infarction.

In one embodiment, in the agent, composition, or kit, the myocardial infarction may be early-onset myocardial infarction.

In one embodiment, in the agent, composition, or kit, the myocardial infarction may be early-onset acute myocardial infarction.

As mentioned above, the early onset means that the disease occurred under the age of 50 for men and under 60 years of age for women.

In one embodiment, the kit may further include an agent for detecting genetic mutations (genetic loci) other than the novel genetic markers described above.

In another aspect, exemplary embodiments of the present invention provide rs1277393322, rs10810978, rs1351282285, rs1560389462, rs10235820, rs2323404, rs7641082, rs8009869, rs1405402, rs1918 from a sample. 101, rs7641013, rs10232190, rs200715251, rs1918100, rs9855437, rs941068, rs6770247, rs1526719 , rs80334730, rs77800378, rs12487132, rs9873508, rs1526708, rs1958821, rs591012, rs1526709, rs200514416, rs111432322, rs34330766, rs7 638747, rs10589173, rs12639020, rs12639023, rs239576, rs7759915, rs372341820, rs78631167, rs527249040, rs184610791, rs1614576, rs16575 38, rs1657545, rs240224 , rs7232479, rs13099537, rs152042, rs131570, rs7191762, rs4584426, rs152041, rs11649332, rs147169123, rs55819522, rs6573071, rs124477 63, rs2520017, rs2520019, rs11642116, rs7196602, rs2334246, rs194817, rs168974, rs183172, rs2152884, rs141073026, rs200261514, rs5072, rs109592 , rs56265975, rs12438548, rs199830494, rs113612782, rs187748, rs174217, rs2520009, rs194797, rs117684941, rs4901620, rs12921822, rs19 Detecting one or more polymorphic sites selected from the group consisting of 4800, rs10852254, rs194815, rs194813, rs174219 and rs9357455 Including, a method of providing information for predicting or diagnosing myocardial infarction or a method of calculating the risk of myocardial infarction is provided.

In one embodiment, the detection is performed using an allele-specific probe hybridization method, an allele-specific amplification method, a sequencing method, or a 5' nuclease digestion method ( 5' nuclease digestion, molecular beacon assay, oligonucleotide ligation assay, size analysis, and single-stranded conformation polymorphism. It may be performed by any one or more methods selected from the group.

In one embodiment, the sample may be a biological sample separated from a diagnostic subject. In a non-limiting example, the sample includes, but is not limited to, one or more selected from tissues, cells, body fluids, feces, urine, plasma, serum, whole blood, cells isolated from blood, cell-free polynucleotides, etc.

In one embodiment, as can be seen in the examples below, rs1614576, rs1657538, rs1657545, rs152042, rs7191762, rs152041, rs11649332, rs12447763, rs2520017, rs2520019, rs11642 116, rs7196602, rs2334246, rs194817, rs168974, rs183172, rs109592, rs56265975 , rs113612782, rs187748, rs174217, rs2520009, rs194797, rs194800, rs10852254, rs194815, rs194813 and rs174219 may at least be polymorphisms associated with thrombosis, but excluding involvement in other functions. That is not the case.

In one embodiment, as can be seen in the following examples, rs78631167 may be a polymorphism related to at least fibrinolysis, but it is not excluded that it is related to other functions.

In one embodiment, as can be seen in the following examples, rs10810978, rs7759915, rs5072, and rs117684941 may be at least polymorphisms related to lipid metabolism, but are not excluded from being related to other functions.

In one embodiment, as can be seen in the examples below, rs8009869, rs80334730, rs77800378, rs1958821, rs111432322, rs6573071, rs4901620, and rs9357455 may at least be polymorphisms related to inflammation, but are excluded from being related to other functions. It's not like that.

Hereinafter, the configuration and effects of the present invention will be described in more detail through examples. However, the examples below are provided only for illustrative purposes to aid understanding of the present invention, and the scope and scope of the present invention are not limited thereto.

[Example 1] Selection of SNPs associated with myocardial infarction

1. Subject selection

596 patients with early-onset acute myocardial infarction from four teaching hospitals in Korea and 643 healthy patients from the Korean Genome Project (KGP) were enrolled as subjects in a study according to an embodiment of the present invention. The patients with early-onset acute myocardial infarction were defined as patients with acute myocardial infarction under 50 years of age for men and under 60 years of age for women. Written informed consent was obtained from all subjects, and sample collection and sequencing were approved by the Institutional Review Board (IRB) of Ulsan National Institute of Science and Technology (UNISTIRB-15-19-A). The subjects' characteristics related to myocardial infarction are shown in Figure 1. In Figure 1, Early-onset AMI refers to patients with acute myocardial infarction, and Control refers to healthy subjects.

2. Whole-genome sequencing (WGS) by Illumina NovaSeq sequencer

WGS was performed with the Illumina NovaSeq 6000 platform and clinical information was matched from KGP data. Genomic DNA was isolated from the plates using the DNeasy Blood & Tissue kit (Qiagen, Germany) according to the manufacturer's protocol. Extracted DNA was quantified using the Quant-iT BR assay kit (Invitrogen), and high molecular weight genomic DNA was sheared using a Covaris S2 ultra sonicator system to obtain appropriately sized fragments. Libraries with short 350-base pair (bp) inserts for paired-end reads were prepared using the TruSeq Nano DNA sample preparation kit according to the manufacturer's protocol for Illumina-based sequencing. Quantification was performed using the Bioanalyzer 2100 (Agilent, Santa Clara, CA, USA), and raw data were generated using the Illumina NovaSeq 6000 platform (Illumina). Information about KGP data can be found on the Korea Genome Project website (http://koreangenome.org). Clusters were generated using paired-end 2Х 150-bp cycle sequencing reads through resequencing.

3. Genome-wide association study (GWAS)

GWAS was performed using logistic regression in an additive genetic model using PLINK (ver. 1.9b). A total of 7,869,081 single nucleotide polymorphisms (SNPs) and insertions/deletions (indels) were tested. Gender and the top 10 major factors were included in the model as covariates. The genome-wide putative threshold was determined to be 1 Х 10 ^-5 for the putative variant. Putative variants were considered new according to the following criteria:

(1) SNVs that do not overlap with previously reported loci for myocardial infarction.

(2) SNVs whose lead variants do not have LD variants (r ² > 0.1) at loci previously reported for myocardial infarction.

Variants were grouped into loci using PLINK (ver. 1.9b) using the ‘--clump-r2 0.1 -clump-window-size 250’ option.

3. Quantitative trait loci (QTL) mapping

Variants were mapped to expression QTL (eQTL), splicing QTL (sQTL), and methylation QTL (mQTL) using publicly available data sets. For eQTLs that explain a portion of the genetic variation in gene expression phenotypes, key variants from GWAS were mapped to eQTLs in the GTEx and eQTLGen datasets. For sQTL, we used the GTEx data set, and for mQTL, we used mQTLdb, a large-scale genome-wide DNA methylation analysis of 1,000 mother-child pairs at serial time points over the life course. QTL for putative read variants were reported.

4. A new genomic locus associated with myocardial infarction

From GWAS, we identified 29 novel genomic loci (85 variants) for acute myocardial infarction that exceeded the genome-wide estimated cutoff (P-value cutoff = 1 Х 10 ^-5 ) (Figures 2A and 3).

Among these, a locus related to thrombosis and fibrinolysis was identified, which was rs1614576, located upstream of PRKCB, which had a putative association (OR = 1.646, P = 3.41 Х 10 ^-6 ) (Figure 2b). . It involves platelet reactions that are associated with the formation of blood clots. rs78631167 is another novel locus located upstream of PLAUR (Plasminogen activator, urokinase receptor) (OR = 0.4725, P = 2.93 Х 10 ^-6 ) and is associated with fiprinolysis (Fig. 2c). rs78631167 was predicted to be located in a regulatory region with a RegulomeDB rank of 4, representing a transcription factor (TF) and DNase peak site. Additionally, a new locus related to inflammation and lipid metabolism, rs9357455, was discovered, which was located upstream of PHACTR1 (Phosphatase and actin regulator 1) and showed a novel putative association (OR = 0.6658, P = 9.73 Х 10 ^-6) (Figure 2d). It was predicted to have a regulation function with a RegulomeDB rank of 5. It also regulates oxidative stress and inflammation in coronary artery endothelial cells through interaction with NF-kB/p65. Additionally, a new mutation called rs9357455 in PHACTR1 was found to be associated with acute myocardial infarction (Figure 2D). A genetic risk locus for acute myocardial infarction was identified, rs5072 (OR = 1.545, P = 8.61 Х 10 ^-6 ), located in the intron of APOA1-AS (Apolipoprotein A1 antisense RNA), which is involved in lipid metabolism (Figure 2e). It regulates the expression of APOA1, whose protein is a component of HDL cholesterol and a key participant in the regulation of reverse cholesterol transport from peripheral tissues to the liver.

Specifically, information on the 85 myocardial infarction-specific genetic markers and the new 29 loci and functions obtained in one embodiment of the present invention is shown in Tables 1 to 12. In Tables 1 to 12, gene items are indicated by the genes preceding and following the mutation (for example, geneA-geneB), and when indicated as NA, it means that the surrounding genes are far away.

number rs ID gene gene function Chromosome location on chromosome One rs1277393322 FRG1CP-FRG1DP Unknown 20 28,772,995 2 rs10810978 ADAMTSL1 Lipid metabolism 9 18,523,845 3 rs1351282285 N.A. Unknown 3 164,704,630 4 rs1560389462 MUC4 Cell adhesion 3 195,788,126 5 rs10235820 PDE1C VSMC proliferation 7 32,082,944 6 rs2323404 LINC02005-CNTN3 Unknown 3 73,926,364 7 rs7641082 LINC02005-CNTN3 Unknown 3 73,923,420 8 rs8009869 LINC00520-PELI2 Ubiquitin ligase activity, inflammation 14 55,900,262 9 rs1405402 LINC02005-CNTN3 Unknown 3 73,921,969 10 rs1918101 LINC02005-CNTN3 Unknown 3 73,927,087 11 rs7641013 LINC02005-CNTN3 Unknown 3 73,923,383 12 rs10232190 KMT2C Histone methyltransferase, cardiomyopathy 7 152,231,944 13 rs200715251 GOLGA8T-LINC02249 Unknown 15 30,175,826 14 rs1918100 LINC02005-CNTN3 Unknown 3 73,927,219 15 rs9855437 LINC02005-CNTN3 Unknown 3 73,925,188 16 rs941068 LINC02005-CNTN3 Unknown 3 73,925,641 17 rs6770247 LINC02005-CNTN3 Unknown 3 73,927,363 18 rs1526719 LINC02005-CNTN3 Unknown 3 73,927,320 19 rs80334730 LINC00520-PELI2 Ubiquitin ligase activity, inflammation 14 55,906,845 20 rs77800378 LINC00520-PELI2 Ubiquitin ligase activity, inflammation 14 55,907,084

number Freeze reference
(Reference allele) Alternative Allyll
(Alternative allele) Freeze effect
(Effect allele) One G A A 2 C A C 3 TTAAATG T T 4 GGGTGGTGTGACCTGTGGATACTGAGGAAGTGTCGGTGACAGGAAGAGAGGTGGCGTGACCTGTGGATGCTGAGGAAGTGTCGGTGACAGGAAGAGGGGTGGTGTGACCTGTGGATACTGAGGAAGTGTCGGTGACAGGAAGAGA G G 5 A G A 6 A G A 7 T C T 8 A G G 9 G A G 10 G T G 11 T C T 12 G A A 13 A G G 14 T A T 15 A G A 16 C T C 17 G A G 18 A G G 19 T C C 20 G A A

number mutation type P-value Odds Ratio In the myocardial infarction group
Genetic mutation frequency In the control group
Genetic mutation frequency One Intergenic variant (IGR) 3.36E-18 5.713 0.1398 0.03571 2 Intron 1.94E-14 0.4509 0.3486 0.5009 3 IGR 5.67E-10 0.2394 0.02517 0.0891 4 In_Frame_Del 1.31E-08 0.2562 0.02336 0.07353 5 Intron 2.21E-08 0.497 0.1416 0.2302 6 IGR 1.98E-07 1.606 0.532 0.431 7 IGR 4.08E-07 1.585 0.5242 0.4267 8 IGR 4.49E-07 1.653 0.3523 0.2733 9 IGR 4.81E-07 1.579 0.5311 0.4328 10 IGR 5.47E-07 1.576 0.5302 0.4328 11 IGR 5.92E-07 1.574 0.5233 0.4267 12 Intron 6.24E-07 1.98 0.171 0.106 13 IGR 6.56E-07 1.84 0.2271 0.1477 14 IGR 7.45E-07 1.764 0.2522 0.169 15 IGR 9.60E-07 1.754 0.2504 0.1681 16 IGR 1.08E-06 1.748 0.2513 0.169 17 IGR 1.08E-06 1.748 0.2513 0.169 18 IGR 1.20E-06 1.745 0.2478 0.1664 19 IGR 1.22E-06 1.615 0.3541 0.2784 20 IGR 1.22E-06 1.615 0.3541 0.2784

number rs ID gene gene function Chromosome location on chromosome 21 rs12487132 LINC02005-CNTN3 Unknown 3 73,919,134 22 rs9873508 LINC02005-CNTN3 Unknown 3 73,925,782 23 rs1526708 LINC02005-CNTN3 Unknown 3 73,918,804 24 rs1958821 LINC00520-PELI2 Ubiquitin ligase activity, inflammation 14 55,908,821 25 rs591012 TTK Cell cycle regulation 6 80,038,900 26 rs1526709 LINC02005-CNTN3 Unknown 3 73,918,900 27 rs200514416 C9orf170-DAPK1 Apoptosis 9 87,414,203 28 rs111432322 LINC00520-PELI2 Ubiquitin ligase activity, inflammation 14 55,905,697 29 rs34330766 LINC02005-CNTN3 Unknown 3 73,924,589 30 rs7638747 LINC02005-CNTN3 Unknown 3 73,923,365 31 rs10589173 N.A. Unknown 14 55,905,174 32 rs12639020 LINC02005-CNTN3 Unknown 3 73,919,588 33 rs12639023 LINC02005-CNTN3 Unknown 3 73,919,636 34 rs239576 TTK Cell cycle regulation 6 80,021,249 35 rs7759915 TTK-BCKDHB Cell cycle regulation, lipid metabolism 6 80,062,270 36 rs372341820 SMG1P2-SPN T cell function, immune response 16 29,655,837 37 rs78631167 PLAUR-IRGC Fibrinolysis 19 43,676,115 38 rs527249040 CNN2 Smooth muscle contraction 19 1,029,328 39 rs184610791 MIR3937-MIR1587 Unknown X 39,788,017 40 rs1614576 ERN2-CHP2 Thrombosis 16 23,747,804

number Freeze reference
(Reference allele) Alternative Allyll
(Alternative allele) Freeze effect
(Effect allele) 21 A C A 22 G A G 23 G A G 24 G C C 25 G A G 26 C A C 27 T C C 28 C T T 29 A G A 30 A G A 31 ATATAT A A 32 C T C 33 C T C 34 G A G 35 C T T 36 G A A 37 T C C 38 G C C 39 C G G 40 A G G

number mutation type P-value Odds Ratio In the myocardial infarction group
Genetic mutation frequency In the control group
Genetic mutation frequency 21 IGR 1.26E-06 1.747 0.247 0.1655 22 IGR 1.33E-06 1.74 0.2504 0.169 23 IGR 1.34E-06 1.744 0.2478 0.1672 24 IGR 1.44E-06 1.614 0.3523 0.2776 25 Intron 1.47E-06 0.5831 0.1632 0.2439 26 IGR 1.59E-06 1.736 0.2487 0.1681 27 IGR 1.78E-06 1.948 0.1658 0.1009 28 IGR 1.83E-06 1.601 0.3515 0.2767 29 IGR 1.88E-06 1.731 0.2444 0.1647 30 IGR 1.97E-06 1.728 0.2461 0.1672 31 5'Flank 2.02E-06 1.598 0.3515 0.2776 32 IGR 2.19E-06 1.722 0.2487 0.169 33 IGR 2.19E-06 1.722 0.2487 0.169 34 Intron 2.41E-06 0.589 0.1632 0.2422 35 IGR 2.41E-06 0.589 0.1632 0.2422 36 IGR 2.75E-06 0.1804 0.008636 0.03879 37 IGR 2.93E-06 0.4725 0.06304 0.1129 38 Intron 3.20E-06 0.2916 0.01903 0.05948 39 IGR 3.23E-06 0.2344 0.02065 0.08382 40 IGR 3.41E-06 1.646 0.2668 0.1931

number rs ID gene gene function Chromosome location on chromosome 41 rs1657538 ERN2-CHP2 Thrombosis 16 23,747,877 42 rs1657545 ERN2-CHP2 Thrombosis 16 23,748,316 43 rs240224 TTK Cell cycle regulation 6 80,007,571 44 rs7232479 LOC644669-NONE Unknown 18 15,377,667 45 rs13099537 LINC02005-CNTN3 Unknown 3 73,923,060 46 rs152042 CHP2 Thrombosis 16 23,754,252 47 rs131570 DUXAP8-CCT8L2 Protein folding 22 16,400,343 48 rs7191762 ERN2-CHP2 Thrombosis 16 23,741,456 49 rs4584426 OR2T8 Olfactory receptor One 247,921,552 50 rs152041 CHP2 Thrombosis 16 23,754,034 51 rs11649332 ERN2-CHP2 Thrombosis 16 23,748,912 52 rs147169123 IZUMO3-TUSC1 Unknown 9 25,189,022 53 rs55819522 N.A. Unknown 16 23,771,655 54 rs6573071 LINC00520-PELI2 Ubiquitin ligase activity, inflammation 14 55,904,081 55 rs12447763 ERN2-CHP2 Thrombosis 16 23,742,273 56 rs2520017 CHP2-PRKCB Thrombosis 16 23,784,944 57 rs2520019 CHP2-PRKCB Thrombosis 16 23,785,567 58 rs11642116 CHP2-PRKCB Thrombosis 16 23,786,091 59 rs7196602 CHP2-PRKCB Thrombosis 16 23,786,294 60 rs2334246 CHP2-PRKCB Thrombosis 16 23,787,611

number Freeze reference
(Reference allele) Alternative Allyll
(Alternative allele) Freeze effect
(Effect allele) 41 G A A 42 A G G 43 G T G 44 G A A 45 T C T 46 A G G 47 T C C 48 G A A 49 A G G 50 G C C 51 C T T 52 A AT A 53 TAA T T 54 G A A 55 G T T 56 G A A 57 T C C 58 A C C 59 C T T 60 A T T

number mutation type P-value Odds Ratio In the myocardial infarction group
Genetic mutation frequency In the control group
Genetic mutation frequency 41 IGR 3.41E-06 1.646 0.2668 0.1931 42 IGR 3.41E-06 1.646 0.2668 0.1931 43 Intron 3.45E-06 0.5943 0.1641 0.2422 44 IGR 3.82E-06 1.763 0.2418 0.1569 45 IGR 4.17E-06 1.696 0.2461 0.169 46 5'Flank 4.52E-06 1.635 0.266 0.1922 47 IGR 4.66E-06 0.5444 0.1097 0.1724 48 IGR 4.82E-06 1.659 0.2444 0.1741 49 Missense_Mutation 4.83E-06 1.538 0.3782 0.2851 50 5'Flank 4.93E-06 1.632 0.266 0.1931 51 IGR 4.98E-06 1.632 0.2627 0.1887 52 IGR 5.14E-06 0.5226 0.09585 0.15 53 IGR 6.41E-06 1.624 0.2651 0.1931 54 IGR 6.72E-06 1.531 0.4016 0.3302 55 IGR 7.60E-06 1.661 0.2332 0.1638 56 IGR 7.94E-06 1.616 0.2642 0.1931 57 IGR 7.94E-06 1.616 0.2642 0.1931 58 IGR 7.94E-06 1.616 0.2642 0.1931 59 IGR 7.94E-06 1.616 0.2642 0.1931 60 IGR 7.94E-06 1.616 0.2642 0.1931

number rsID gene gene function Chromosome location on chromosome 61 rs194817 CHP2-PRKCB Thrombosis 16 23,788,500 62 rs168974 CHP2-PRKCB Thrombosis 16 23,789,042 63 rs183172 CHP2-PRKCB Thrombosis 16 23,789,509 64 rs2152884 RYR2 Calcium signaling, cardiomyopathy One 237,214,855 65 rs141073026 TM2D1 Apoptosis One 61,717,206 66 rs200261514 LINC02444-LOC100507377 Unknown 12 73,222,956 67 rs5072 APOA1-AS Lipid metabolism 11 116,836,867 68 rs109592 CHP2 Thrombosis 16 23,757,389 69 rs56265975 CHP2 Thrombosis 16 23,759,927 70 rs12438548 MIR4510-C15orf41 Unknown 15 36,119,067 71 rs199830494 LINC01243-ACO1 Enzyme in the TCA cycle 9 32,154,607 72 rs113612782 CHP2-PRKCB Thrombosis 16 23,761,303 73 rs187748 CHP2-PRKCB Thrombosis 16 23,767,186 74 rs174217 CHP2-PRKCB Thrombosis 16 23,768,995 75 rs2520009 CHP2-PRKCB Thrombosis 16 23,769,092 76 rs194797 CHP2-PRKCB Thrombosis 16 23,769,518 77 rs117684941 PIK3C2G PI3K-AkT signaling, glucose and lipid metabolism 12 18,556,791 78 rs4901620 LINC00520-PELI2 Ubiquitin ligase activity, inflammation 14 55,901,317 79 rs12921822 RBFOX1 Cardiomyopathy 16 7,002,773 80 rs194800 CHP2-PRKCB Thrombosis 16 23,763,247 81 rs10852254 CHP2-PRKCB Thrombosis 16 23,790,378 82 rs194815 CHP2-PRKCB Thrombosis 16 23,790,834 83 rs194813 CHP2-PRKCB Thrombosis 16 23,791,390 84 rs174219 CHP2-PRKCB Thrombosis 16 23,791,599 85 rs9357455 LINC02530-PHACTR1 Inflammation 6 12,693,654

number Freeze reference
(Reference allele) Alternative Allyll
(Alternative allele) Freeze effect
(Effect allele) 61 G A A 62 T A A 63 T C C 64 G A A 65 A C C 66 G GTAAT GTAAT 67 A G A 68 C T T 69 T G G 70 G A G 71 G A G 72 G A A 73 G A A 74 A G G 75 C T T 76 T C C 77 T C C 78 G A A 79 C T C 80 T C C 81 T C C 82 A G G 83 T C C 84 T C C 85 C T C

number mutation type P-value Odds Ratio In the myocardial infarction group
Genetic mutation frequency In the control group
Genetic mutation frequency 61 IGR 7.94E-06 1.616 0.2642 0.1931 62 IGR 7.94E-06 1.616 0.2642 0.1931 63 IGR 7.94E-06 1.616 0.2642 0.1931 64 Intron 8.02E-06 1.53 0.4361 0.3534 65 Intron 8.13E-06 1.673 0.2219 0.1552 66 IGR 8.25E-06 2.644 0.07168 0.03109 67 Intron 8.61E-06 1.545 0.3817 0.3078 68 Intron 8.63E-06 1.609 0.266 0.1948 69 3'Flank 8.63E-06 1.609 0.266 0.1948 70 IGR 8.72E-06 0.6094 0.2133 0.2707 71 IGR 8.77E-06 0.6313 0.199 0.2772 72 IGR 8.92E-06 1.61 0.2651 0.194 73 IGR 8.92E-06 1.61 0.2651 0.194 74 IGR 8.92E-06 1.61 0.2651 0.194 75 IGR 8.92E-06 1.61 0.2651 0.194 76 IGR 8.92E-06 1.61 0.2651 0.194 77 Intron 8.95E-06 0.2487 0.01295 0.04397 78 IGR 8.96E-06 1.523 0.4024 0.3328 79 Intron 9.05E-06 1.601 0.2694 0.1888 80 IGR 9.09E-06 1.611 0.2642 0.1931 81 IGR 9.12E-06 1.605 0.2668 0.1957 82 IGR 9.12E-06 1.605 0.2668 0.1957 83 IGR 9.12E-06 1.605 0.2668 0.1957 84 IGR 9.12E-06 1.605 0.2668 0.1957 85 IGR 9.73E-06 0.6658 0.3808 0.475

5. QTL (Quantitative Trait Loci) mapping of new loci

Of the 29 lead variants, 14 tended to have larger effect sizes compared to European (UK biobank; http://www.nealelab.is/uk-biobank/) and Japanese MI (Biobank of Japan) studies. was confirmed (Figure 3). The remaining read mutations were not reported in conventional SNP chip-based studies. Among the 29 novel loci for early-onset acute myocardial infarction, 5 loci were found to be eQTL based on the GTEx database ( Fig. 4A ). Whole blood (eQTL Bonferroni adjusted P = 4 Х 10 ^-207 ) by the Rs1614576 eQTLGen database located upstream of PRKCB and artery tibial (P = 2.75 Х 10 ^-14 ; Fig. 4b) and artery aorta (P = 1.22 Х 10 ) by the GTEx database. ^-9 ) showed the most significant qQTL signal. Rs591012, located in the TTK gene, is not only a qQTL (P = 4.34 Х 10 ^-17 in artery tibial; Figure 4c) affecting the expression of ELOVL4 (ELOVL fatty acid elongase 4), which is involved in lipid metabolism, but also an alternative splicing factor for the gene. It was an sQTL that changes alternative splicing. Rs5072, located in APOA1-AS, was associated with AFAH1B2 (platelet activating factor acetylhydrolase 1b catalytic subunit 2) (P = 1.68 Х 10 ^-4 ; Figure 4d) and PCSK7 (proprotein convertase subtilisin/kexin type 7) ( P = 3.96 Х 10 ^-11 ) showed an eQTL signal changing the expression. PAFAH1B2 encodes a subunit of PAFAH that degrades and inactivates platelet-activating factor (PAF). Additionally, rs10232190 affected the expression of LINC01103 (P = 1.00 Х 10 ^-6 in heart atrial appendage, P = 1.16 Х 10 ^-6 in whole blood, Figure 4e). LINC01103 can change the expression of PIM1 (proto-oncogene serine/threonine-protein kinase Pim-1), and inhibition of PIM1 inhibits VSMC proliferation and the development of atherosclerosis.

Although exemplary embodiments of the present invention have been described above in relation to the above-mentioned preferred embodiments, various modifications and variations can be made without departing from the gist and scope of the invention. Accordingly, the appended claims will include such modifications and variations as long as they fall within the spirit of the present invention.

Claims (8)

rs1277393322, rs10810978, rs1351282285, rs1560389462, rs10235820, rs2323404, rs7641082, rs8009869, rs1405402, rs1918101, rs7641013, rs10232190, rs200715251, rs1918100, rs9855437, rs941068, rs6770247, rs1526719, rs80334730, rs77800378, rs12487132, rs9873508, rs1526708 , rs1958821, rs591012, rs1526709, rs200514416, rs111432322, rs34330766, rs7638747, rs10589173, rs12639020, rs12639023, rs239576, rs7759915, rs372341820, rs7 8631167, rs527249040, rs184610791, rs1614576, rs1657538, rs1657545, rs240224, rs7232479, rs13099537, rs152042, rs131570, rs7191762, rs4 584426, rs152041, rs11649332, rs147169123, rs55819522, rs6573071, rs12447763, rs2520017, rs2520019, rs11642116, rs7196602, rs2334246, rs194817, rs16897 4, rs183172, rs2152884, rs141073026, rs200261514, rs5072, rs109592, rs56265975, rs12438548, rs199830494, rs113612782, rs187748, rs17421 7, rs2520009, A polynucleotide containing one or more polymorphisms selected from the group consisting of rs194797, rs117684941, rs4901620, rs12921822, rs194800, rs10852254, rs194815, rs194813, rs174219 and rs9357455, or complementary thereto Myocardium comprising an agent that detects a polynucleotide of the sequence Composition for predicting or diagnosing infarction. According to paragraph 1,
A composition wherein the agent comprises a primer pair or probe that specifically binds to the polynucleotide or a polynucleotide of a sequence complementary thereto. According to paragraph 2,
The composition, wherein the probe is an oligonucleotide probe, a single stranded DNA probe, a double stranded DNA probe, or an RNA probe. According to paragraph 1,
The composition of claim 1, wherein the agent comprises an antibody that detects a polypeptide encoded by the polynucleotide. A kit for predicting or diagnosing myocardial infarction, comprising the composition of any one of claims 1 to 4. From samples rs1277393322, rs10810978, rs1351282285, rs1560389462, rs10235820, rs2323404, rs7641082, rs8009869, rs1405402, rs1918101, rs7641013 , rs10232190, rs200715251, rs1918100, rs9855437, rs941068, rs6770247, rs1526719, rs80334730, rs77800378, rs12487132, rs9873508, rs15267 08, rs1958821, rs591012, rs1526709, rs200514416, rs111432322, rs34330766, rs7638747, rs10589173, rs12639020, rs12639023, rs239576, rs7759915, rs3723 41820, rs78631167, rs527249040, rs184610791, rs1614576, rs1657538, rs1657545, rs240224, rs7232479, rs13099537, rs152042, rs131570, rs71 91762,rs4584426, rs152041, rs11649332, rs147169123, rs55819522, rs6573071, rs12447763, rs2520017, rs2520019, rs11642116, rs7196602, rs2334246, rs19481 7, rs168974, rs183172, rs2152884, rs141073026, rs200261514, rs5072, rs109592, rs56265975, rs12438548, rs199830494, rs113612782, rs18774 8, rs174217, One or more polymorphic sites selected from the group consisting of rs2520009, rs194797, rs117684941, rs4901620, rs12921822, rs194800, rs10852254, rs194815, rs194813, rs174219 and rs9357455. Method for providing information for predicting or diagnosing myocardial infarction, including the step of detecting . According to clause 6,
The detection is performed using an allele-specific probe hybridization method, an allele-specific amplification method, a sequencing method, a 5' nuclease digestion method, a molecular beacon assay, an oligonucleotide binding assay, a size analysis method, and a single-strand conformational polymorphism method. A method of providing information for predicting or diagnosing myocardial infarction, performed by one or more methods selected from the group consisting of. According to clause 6,
The sample is information for predicting or diagnosing myocardial infarction, including any one or more selected from the group consisting of tissues, cells, body fluids, stool, urine, plasma, serum, whole blood, cells isolated from blood, and cell-free polynucleotides. How to provide.