The Branched-chain Amino Acid Transaminase 1 -23C/G Polymorphism Confers Protection Against Acute Coronary Syndrome

Ramírez-Bello, Julian; Vargas-Alarcón, Gilberto; Pérez-Méndez, Óscar; Martínez-Ríos, Marco A.; Peña-Duque, Marco A.; Cardoso-Saldaña, Guillermo; Posadas-Romero, Carlos; Sierra-Martínez, Mónica; Fragoso, José M.; Ramírez-Bello, Julian; Vargas-Alarcón, Gilberto; Pérez-Méndez, Óscar; Martínez-Ríos, Marco A.; Peña-Duque, Marco A.; Cardoso-Saldaña, Guillermo; Posadas-Romero, Carlos; Sierra-Martínez, Mónica; Fragoso, José M.

doi:10.24875/ric.19003133

Servicios Personalizados

Revista

Articulo

Indicadores

Citado por SciELO
Accesos

Links relacionados

Similares en SciELO

Otros
Otros

Permalink

Revista de investigación clínica

versión On-line ISSN 2564-8896versión impresa ISSN 0034-8376

Rev. invest. clín. vol.72 no.1 Ciudad de México ene./feb. 2020 Epub 04-Mayo-2021

https://doi.org/10.24875/ric.19003133

Original articles

The Branched-chain Amino Acid Transaminase 1 -23C/G Polymorphism Confers Protection Against Acute Coronary Syndrome

Julian Ramírez-Bello¹^*

Gilberto Vargas-Alarcón²

Óscar Pérez-Méndez²

Marco A. Martínez-Ríos³

Marco A. Peña-Duque³

Guillermo Cardoso-Saldaña⁴

Carlos Posadas-Romero⁴

Mónica Sierra-Martínez⁵

José M. Fragoso²

^¹Research Unit, Hospital Juárez de México, Mexico City, Mexico

^²Department of Molecular Biology, Instituto Nacional de Cardiología Ignacio Chávez, Mexico City, Mexico

^³Department of Interventional Cardiology and Instituto Nacional de Cardiología Ignacio Chávez, Mexico City, Mexico

^⁴Department of Endocrinology, Instituto Nacional de Cardiología Ignacio Chávez, Mexico City, Mexico

^⁵Department of Laboratory of Genetics and Molecular Diagnosis, Hospital Juárez de México, Mexico City, Mexico

ABSTRACT

Background:

Previous studies have shown an association between polymorphisms of the BAT1-NF-κB inhibitor-like-1 (NFKBIL1)-LTA genomic region and susceptibility to myocardial infarction and acute coronary syndrome (ACS).

Objective:

The objective of the study was to study the role of three polymorphisms in the BAT1, NFKBIL1, and LTA genes on the susceptibility or protection against ACS; we included a group of cases-controls from Central Mexico.

Methods:

The BAT1 rs2239527C/G, NFKBIL1 rs2071592T/A, and LTA rs1800683G/A polymorphisms were genotyped using a 5’ TaqMan assay in a group of 625 patients with ACS and 617 healthy controls.

Results:

Under a recessive model, the BAT1 -23C/G (rs2239527) polymorphism showed an association with protection against ACS (odds ratio = 0.56, and p-corrected = 0.019). In contrast, the genotype and allele frequencies of the NFKBIL1 rs2071592T/A and LTA rs1800683G/A polymorphisms were similar between ACS patients and controls and no association was identified.

Conclusion:

Our data suggest an association between the BAT1 -23C/G polymorphism and protection against ACS in Mexican patients.

Key words: Acute coronary syndrome; BAT; Single-nucleotide polymorphism

INTRODUCTION

Atherosclerosis is a complex chronic disease of the arterial wall with multifactorial etiology and is the etiological basis of most cardiovascular events, including coronary artery disease (CAD)¹,². Acute coronary syndrome (ACS) comprises a spectrum of obstructive CAD which most commonly arises from plaque rupture and/or erosion, leaving the vulnerable lipid-rich core exposed to the circulation, resulting in activation of platelets, and the coagulation cascade leading to acute thrombotic occlusion. There are three major subtypes of ACS: unstable angina, non-ST-elevation myocardial infarction (NSTEMI), and STEMI. Each subtype represents a different stage in the spectrum of disease. Plaque erosion with subendocardial ischemia represents the majority of cases of unstable angina and NSTEMI, while plaque rupture and complete thrombotic occlusion, of an epicardial coronary, with associated transmural infarction, are characteristic of STEMI³,⁴. A growing body of evidence suggests that the genetic component is an important risk factor for ACS. In this way, some studies have identified an association between single-nucleotide polymorphisms (SNPs) located in branched-chain amino acid transaminase 1 (BAT1), NF-κB inhibitor-like-1 (NFKBIL1) and/or lymphotoxin alpha (LTA) and MI or CAD⁵-⁸. A first study conducted in Japanese population identified an association between various BAT1, NFKBIL1 and LTA single nucleotide polymorphisms (SNPs) polymorphisms, and MI susceptibility. For example, the BAT1 -23G/C (rs2239527), NFKBIL1 -63T/A (rs2071592), and LTA -162G/A (rs1800683 or 10G/A) SNPs showed similar odds ratio (OR) (1.6), 95% confidence interval (CI) (1.25-2.03), and p-value (≈ 0.0004) because they were in high linkage disequilibrium (LD)⁵. In addition, the LTA -162G/A also showed an association with CAD susceptibility (OR 1.2, 95% CI: 1.00-1.50, and p = 0.047) in Chinese population⁸. However, other studies have not replicated these findings⁹-¹². The BAT1, NFKBIL1, and LTA genes are located in the 6p21.3 region. BAT1 encodes a nuclear protein is called HLA-B-associated transcript 1, which negatively regulates the expression of interleukin (IL)-1, tumor necrosis factor (TNF), and IL-6¹³,¹⁴; NFKBIL1 encodes a protein homologous to IκB (κB inhibitors), which regulates the expression of nuclear factor-kappa B transcription factor, TNF, IL-1, and IL-6¹⁵; and LTA encodes a protein involved in the inflammatory and immunological response¹⁶. LTA binds to their cognates, TNF receptors (TNFR1) and TNFR2, and regulates the expression of anti-apoptotic proteins to prevent cell death, inflammatory response, and cell differentiation¹⁷. Thus, these three proteins are involved in various inflammatory processes.

Given the inconsistencies of genetic association between BAT1, NFKBIL1 or LTA, and ACS or MI, our study aimed to determine whether the BAT1 -23C/G, NFKBIL1 -63T/A, and LTA -162G/A polymorphisms (the choice of these variants in these three genes was due to the almost complete LD [≈r²] among them) confer risk or protection against ACS in Mexican patients.

MATERIAL AND METHODS

Subjects

All subjects included in this study were ethnically matched and were considered Mexican Mestizo only those individuals whose families had been born in Mexico for three generations, including their own. A Mexican Mestizo is defined as someone born in Mexico, who is a descendant of the original autochthonous inhabitants of the region, and of individuals of Caucasian (predominantly Spaniards) and/or African origin, who came to the American continent during the 16^th century. The ethnical characteristics of the studied groups were demonstrated analyzing 265 ancestry informative markers (AIMs). The results showed a similar background between patients and controls. Patients showed 55.8%, 34.4%, and 9.8% of Amerindian, Caucasian, and African ancestry, respectively, whereas controls showed 54.1%, 35.8%, and 10.1% of Amerindian, Caucasian, and African ancestry, respectively. Our study included 1242 Mexican Mestizos, 625 (501 men and 124 women, with a mean age of 58.2 ± 10.4 years) patients with ACS and 617 (468 men and 149 women, with a mean age of 54.01 ± 7.69 years) controls (individuals who had no history of ACS or CAD, symptoms or previous diagnosis of cardiovascular disease). Five hundred and two patients presented MI, and 123 had unstable angina. The ACS patients were diagnosed according to the World Health Organization and the American Heart Association/American College of Cardiology criteria¹⁸,¹⁹. Both cases and controls were referred from the Instituto Nacional de Cardiología (INC) Ignacio Chávez, Mexico City. All the patients and controls provided written informed consent. Our study was approved by the Ethics and Research Committee of INC.

DNA extraction

We used the DNA extraction method proposed by Lahiri and Nurnberger²⁰.

Genetic analysis

The BAT1 -23C/G (rs2239527), NFKBIL1 -63T/A (rs2071592), and LTA -162G/A (rs1800683) SNPs were genotyped using a TaqMan SNP genotyping assay on a 7900HT fast real-time polymerase chain reaction system according to manufacturer’s instructions (Applied Biosystems, Foster City, USA). Thermo cycling conditions were as follows: initial denaturation at 95°C for 10 min (1 cycle) followed by 40 cycles at 95°C for 15 sec (denaturation) and at 60°C for 1 min (annealing/extension). Sequenced samples of different genotypes were included as positive controls.

Statistical analysis

The Mann–Whitney U-test was used to compare continuous variables between cases and controls. For categorical variables, we used Chi-square or Fisher’s exact tests. We analyzed the association of the three polymorphisms with ACS by logistic regression and under the codominant, dominant, recessive, over-dominant, and additive genetic models. Multiple logistic models were constructed to identify the variables associated with ACS. p < 0.05 was considered statistically significant. The haplotypes and LD of the BAT1 -23C/G, NFKBIL1 -63T/A, and LTA -162G/A polymorphisms were obtained using the Haploview program (V 4.1, Broad Institute of Massachusetts Institute of Technology and Harvard University, Cambridge, MA, USA). ADMIXTURE software was used to evaluate 265 AIMs in our study population. Hardy-Weinberg equilibrium (HWE) was obtained using Finnet software (https://ihg.gsf.de/cgi-bin/hw/hwa1.pl). Statistical data analysis was performed with SPSS version 18.0 (SPSS, Chicago, Illinois) statistical package.

RESULTS

Characteristics of the study population

Baseline characteristics of the ACS patients and controls included in our study are shown in Table 1. As expected, ACS patients presented a higher frequency of type 2 diabetes (T2D), high blood pressure, dyslipidemia, and smoking habit, and a lower frequency of alcohol habit than controls.

Table 1 Baseline clinical characteristics of the studied individuals

Parameter	β-coefficient	OR	p-value
Clinical characteristics	ACS patients (n[%]) (n=625)	Healthy controls (n[%]) (n=617)	p-value
Men*	501 (80)	468 (76)	NS
High blood pressure (mmHg)	265 (42)	82 (13)	<0.001
Type 2 diabetes mellitus*	189 (42)	63 (14)	<0.001
Dyslipidemia*	288 (46)	216 (35)	<0.001
Smoking*	224 (36)	141 (23)	<0.001
Alcohol*	139 (22)	441 (71)	<0.001
	Median (percentile 25-75)	Median (percentile 25-75)
Age (years)	58 (51-65)	54 (49-59)	0.01
BMI (kg/m²)	27.2 (24.7-29.3)	28.1 (25.4-30.5)	0.01

^*(n[%]) Number and proportion of subjects with the clinical characteristic in both groups.

Genotype frequencies and association analysis

Observed frequencies of the BAT1 -23C/G, NFKBIL1 -63T/A, and LTA -162G/A polymorphisms were in HWE for both cases and controls (p > 0.05). The distribution of the allele and genotype frequencies of NFKBIL1 -63T/A, and LTA -162G/A was similar in cases and controls, and no association was detected (Table 2). Nonetheless, under the genetic recessive model adjusted by gender, age, body mass index (BMI), high blood pressure, T2D, dyslipidemia, alcohol consumption, and smoking habit, the BAT1 -23C/G polymorphism showed an association with protection against ACS (OR = 0.56, 95% CI = 0.35-0.91, and p-corrected = 0.019) (Table 2).

Table 2 Association of the BAT1, NFKBIL1, and LTA SNPs with ACS

Gene and single nucleotide polymorphism	Genotype frequency n (%)			MAF	Model	OR (95%CI)	pC

BAT1 -23 C/G (rs2239527)

Control	CC	CG	GG
(n=617)	272 (44.1)	266 (43.1)	79 (12.8)	0.34	Codominant	0.54 (0.33-0.91)	0.06
					Dominant	0.84 (0.62-1.15)	0.27
					Recessive	0.56 (0.35-0.91)	0.019
ACS	283 (45.2)	281 (45.0)	61 (9.8)	0.32	Heterozygous	1.06 (0.79-1.44)	0.69
(n=625)					Log-additive	0.80 (0.64-1.00)	0.05

NFKBIL1 -63 T/A (rs2071592)

Control	TT	TA	AA

(n=617)	268 (43.4)	275 (44.6)	74 (12.0)	0.34	Codominant	0.68 (0.41-1.13)	0.33
					Dominant	0.87 (0.64-1.19)	0.38
					Recessive	0.71 (0.44-1.14)	0.16
ACS	282 (45.1)	277 (44.3)	66 (10.6)	0.33	Heterozygous	1.01 (0.74-1.36)	0.97
(n=625)					Log-additive	0.86 (0.68-1.08)	0.18

LTA -162 G/A (rs1800683)

Control	GG	GA	AA

(n=617)	260 (42.1)	274 (44.4)	83 (13.5)	0.36	Codominant	0.62 (0.38-1.01)	0.15
					Dominant	0.83 (0.61-1.13)	0.25
					Recessive	0.65 (0.41-1.03)	0.06
ACS	279 (44.6)	276 (44.2)	70 (11.2)	0.33	Heterozygous	1.01 (0.75-1.37)	0.94
(n=625)					Log-additive	0.82 (0.65-1.03)	0.81

ACS: Acute Coronary Syndrome, MAF: minor allele frequency, OR: odds ratio, CI: confidence interval, pC: p-corrected. The p-values were calculated from logistic regression analysis, and the ORs were adjusted for gender, age, body index mass (BMI), high blood pressure, type 2 diabetes, dyslipidemia, alcohol consumption, and smoking. Bold numbers indicate significant associations.

LD analysis

The alleles of the BAT1 -23C/G, NFKBIL1 -63T/A, and LTA -162G/A polymorphisms showed a high LD (r² ≈ 0.9, data not shown). Meanwhile, the distribution of haplotypes was similar between cases and controls, and no association was identified with this inflammatory disease (Table 3).

Table 3 Haplotype (BAT1 -23C/G, NFKBIL1 -63 T/A, and LTA -162 G/A) frequencies (%) in ACS patients and healthy controls

Combination of alleles of the three single nucleotide polymorphisms	ACS (n=625)	Controls (n=617)	Odds ratio	95% Confidence interval	p-value
Haplotype	Hf	Hf
H1 (CTC)	65.3	62.9	1.10	0.94-1.30	0.21
H2 (GAA)	30.6	32.5	0.91	0.77-1.08	0.29
H3 (CAA)	1.4	1.1	1.29	0.62-2.67	0.48

The order of the polymorphisms in the haplotypes is according to the positions in the chromosome (rs2239527, rs2071592, and rs1800683).

Hf: haplotype frequency, ACS: Acute Coronary Syndrome.

DISCUSSION

We analyzed three SNPs located in the BAT1, NFKBIL1, and LTA genes in a group of ACS patients and controls. In the literature, association studies between BAT1 -23C/G, NFKBIL1 -63T/A, and LTA -162G/A and susceptibility or protection to different cardiovascular diseases are scarce and controversial⁵-¹²,²¹. For example, two previous studies showed an association with susceptibility between the LTA -162G/A and A252G polymorphisms and MI in Japanese population⁵,⁶. However, other studies (where only LTA A252G was evaluated) conducted in the same population did not replicate this finding¹⁰,²². In addition, other studies in European-derived populations (patients from Germany and UK), the LTA A252G SNP was not associated with MI susceptibility⁹,¹¹. Contrary to this finding, in another group of ACS patients from Germany, the TCGATCAGA haplotype carrying the BAT -23G, NFKBIL1 -63A, and LTA -162A minor alleles (underlined alleles, respectively) showed an association with protection against MI⁷. Regarding ACS, as far as we know, only one study has been published, and in that report, the authors did not identify any association between LTA A252G and ACS (although a trend toward an association with protection was identified; p = 0.06)¹². Similar to those results, we did not identify any association between this variant and ACS. On the other hand, as far as we know, the NFKBIL1 -63T/A polymorphism has not been evaluated in ACS patients. Our data suggest that this variant is not a risk or protection factor for ACS in the Mexican population. In contrast, we identified an association between the BAT1 -23GG genotype and protection against ACS under the recessive genetic model. As far as we know, this is one of the few studies that describe the association of this polymorphism with protection against ACS. In line with our results, Koch et al. reported that the BAT1 -23GG genotype conferred protection (OR = 0.78) against MI in a German population⁷. In addition, Gnjec et al. reported that the -23 GG genotype of BAT1 -23 C/G was associated with reduced risk of Alzheimer’s disease in Caucasian population (OR = 0.43)²³. On the other hand, Mendonça et al. reported in patients infected with Plasmodium vivax that the -23 G allele was associated with reduced clinical manifestations of malaria in Brazilian populations¹⁴.

A functional study showed that the BAT1 -23G minor allele (we identified an association between the BAT1 -23GG genotype and protection against ACS) affects the binding of OCT1 (a transcription factor) suggesting a biological role of this allele on the BAT1 expression²⁴. That same study showed that the Ying Yang 1 (YY1) transcription factor might bind indirectly with the BAT1 – 23G allele²⁴. OCT1 is ubiquitously expressed in various tissues and cells and can positively or negatively regulate the expression of different genes involved in inflammatory process²⁵, while YY1 suppresses or activates the expression of several genes depending on the features of the promoter or cells²⁴. A previous study reported by Mordvinov et al. showed that the OCT1/YY1 complex is involved in the negative regulation of IL-5 expression in human T cells²⁶; it is possible that this complex leads to a decrease in the expression of other pro-inflammatory cytokine genes.

We recognize that our work has limitations, such as the fact that we studied only one polymorphism in each gene (BAT1, NFKBIL1, and LAT). In addition, the different ancestry of the populations may have biased the association (or no associations) observed between BAT1 -23C/G and ACS. Thus, additional studies in other populations are necessary to understand the role of this variant in ACS. In summary, our data suggest that the NFKBIL1 -63T/A and LTA -162G/A polymorphisms are not risk or protection factors for ACS, while BAT1 -23C/G is associated with protection against ACS in a sample from Mexico.

Finally, our data suggests that BAT1 -23C/G is a protection factor for ACS in Mexican patients.

ACKNOWLEDGMENTS

This study was partially funded by a grant from the Consejo Nacional de Ciencia y Tecnología (CONACyT, Mexico) (FOSISS project number 233277). The authors are grateful to all the participants of this study.

REFERENCES

1. Dzau VJ, Antman EM, Black HR, Hayes DL, Manson JE, Plutzky J, et al. The cardiovascular disease continuum validated:clinical evidence of improved patient outcomes:Part I:pathophysiology and clinical trial evidence (risk factors through stable coronary artery disease). Circulation. 2006;114:2850-70. [ Links ]

2. Libby P. Inflammation in atherosclerosis. Arterioscler Thromb Vasc Biol. 2012;32:2045-51. [ Links ]

3. Dzau VJ, Antman EM, Black HR, Hayes DL, Manson JE, Plutzky J, et al. The cardiovascular disease continuum validated:clinical evidence of improved patient outcomes:Part II:clinical trial evidence (acute coronary syndromes through renal disease) and future directions. Circulation. 2006;114:2871-91. [ Links ]

4. Achar SA, Kundu S, Norcross WA. Diagnosis of acute coronary syndrome. Am Fam Physician. 2005;72:119-26. [ Links ]

5. Ozaki K, Ohnishi Y, Iida A, Sekine A, Yamada R, Tsunoda T, et al. Functional SNPs in the lymphotoxin-alpha gene that are associated with susceptibility to myocardial infarction. Nat Genet. 2002;32:650-4. [ Links ]

6. Iwanaga Y, Ono K, Takagi S, Terashima M, Tsutsumi Y, Mannami T, et al. Association analysis between polymorphisms of the lymphotoxin-alpha gene and myocardial infarction in a Japanese population. Atherosclerosis. 2004;172:197-8. [ Links ]

7. Koch W, Hoppmann P, Michou E, Jung V, Pfeufer A, Mueller JC, et al. Association of variants in the BAT1-NFKBIL1-LTA genomic region with protection against myocardial infarction in Europeans. Hum Mol Genet. 2007;16:1821-7. [ Links ]

8. Liu Y, Sheng H, Lu L, Wu Z, Chen Q, Xiao H, et al. Haplotype-based association of four lymphotoxin-alpha gene polymorphisms with the risk of coronary artery disease in Han Chinese. Tohoku J Exp Med. 2011;224:119-25. [ Links ]

9. Sedlacek K, Neureuther K, Mueller JC, Stark K, Fischer M, Baessler A, et al. Lymphotoxin-alpha and galectin-2 SNPs are not associated with myocardial infarction in two different German populations. J Mol Med (Berl). 2007;85:997-1004. [ Links ]

10. Kimura A, Takahashi M, Choi BY, Bae SW, Hohta S, Sasaoka T, et al. Lack of association between LTA and LGALS2 polymorphisms and myocardial infarction in Japanese and korean populations. Tissue Antigens. 2007;69:265-9. [ Links ]

11. Clarke R, Xu P, Bennett D, Lewington S, Zondervan K, Parish S, et al. Lymphotoxin-alpha gene and risk of myocardial infarction in 6,928 cases and 2,712 controls in the ISIS case-control study. PLoS Genet. 2006;2:e107. [ Links ]

12. Morgan TM, Krumholz HM, Lifton RP, Spertus JA. Nonvalidation of reported genetic risk factors for acute coronary syndrome in a large-scale replication study. JAMA. 2007;297:1551-61. [ Links ]

13. Allcock RJ, Williams JH, Price P. The central MHC gene, BAT1, may encode a protein that down-regulates cytokine production. Genes Cells. 2001;6:487-94. [ Links ]

14. Mendonça VR, Souza LC, Garcia GC, Magalhães BM, Lacerda MV, Andrade BB, et al. DDX39B (BAT1), TNF and IL6 gene polymorphisms and association with clinical outcomes of patients with Plasmodium vivax malaria. Malar J. 2014;13:278. [ Links ]

15. Greetham D, Ellis CD, Mewar D, Fearon U, an Ultaigh SN, Veale DJ, et al. Functional characterization of NF-kappaB inhibitor-like protein 1 (NFkappaBIL1), a candidate susceptibility gene for rheumatoid arthritis. Hum Mol Genet 2007;16:3027-36. [ Links ]

16. Upadhyay V, Fu YX. Lymphotoxin organizes contributions to host defense and metabolic illness from innate lymphoid cells. Cytokine Growth Factor Rev. 2014;25:227-33. [ Links ]

17. Naoum JJ, Chai H, Lin PH, Lumsden AB, Yao Q, Chen C, et al. Lymphotoxin-alpha and cardiovascular disease:clinical association and pathogenic mechanisms. Med Sci Monit. 2006;12:RA121-4. [ Links ]

18. Hamm CW, Bassand JP, Agewall S, Bax J, Boersma E, Bueno H, et al. ESC guidelines for the management of acute coronary syndromes in patients presenting without persistent ST-segment elevation:the task force for the management of acute coronary syndromes (ACS) in patients presenting without persistent ST-segment elevation of the European society of cardiology (ESC). Eur Heart J. 2011;32:2999-3054. [ Links ]

19. Cannon CP, Battler A, Brindis RG, Cox JL, Ellis SG, Every NR, et al. American college of cardiology key data elements and definitions for measuring the clinical management and outcomes of patients with acute coronary syndromes. A report of the American college of cardiology task force on clinical data standards (Acute coronary syndromes writing committee). J Am Coll Cardiol. 2001;38:2114-30. [ Links ]

20. Lahiri DK, Nurnberger JI Jr. A rapid non-enzymatic method for the preparation of HMW DNA from blood for RFLP studies. Nucleic Acids Res. 1991;19:5444. [ Links ]

21. Ryan AW, O'Brien E, Shields D, McManus R. Lack of association between NFKBIL1/LTA polymorphisms and hypertension, myocardial infarct, unstable angina and stable angina in a large Irish population sample. Atherosclerosis. 2008;197:465-6. [ Links ]

22. Yamada A, Ichihara S, Murase Y, Kato T, Izawa H, Nagata K, et al. Lack of association of polymorphisms of the lymphotoxin alpha gene with myocardial infarction in Japanese. J Mol Med (Berl). 2004;82:477-83. [ Links ]

23. Gnjec A, D'Costa KJ, Laws SM, Hedley R, Balakrishnan K, Taddei K, et al. Association of alleles carried at TNFA 850 and BAT1 22 with Alzheimer's disease. J Neuroinflammation. 2008;5:36. [ Links ]

24. Price P, Wong AM, Williamson D, Voon D, Baltic S, Allcock RJ, et al. Polymorphisms at positions 22 and 348 in the promoter of the BAT1 gene affect transcription and the binding of nuclear factors. Hum Mol Genet. 2004;13:967-74. [ Links ]

25. Zhao FQ. Octamer-binding transcription factors:genomics and functions. Front Biosci (Landmark Ed). 2013;18:1051-71. [ Links ]

26. Mordvinov VA, Schwenger GT, Fournier R, De Boer ML, Peroni SE, Singh AD, et al. Binding of YY1 and oct1 to a novel element that downregulates expression of IL-5 in human T cells. J Allergy Clin Immunol. 1999;103:1125-35. [ Links ]

Received: June 03, 2019; Accepted: September 02, 2019

^* Corresponding author: Julian Ramírez-Bello E-mail: dr.julian.ramirez.hjm@gmail.com

Instituto Nacional de Cardiología Ignacio Chávez. Published by Permanyer. This is an open ccess article under the CC BY-NC-ND license