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CREB1是定期运动时运动心率反应变化的一个强有力的基因预测指标:遗产家庭研究。

CREB1 is a strong genetic predictor of the variation in exercise heart rate response to regular exercise: the HERITAGE Family Study.

作者信息

Rankinen Tuomo, Argyropoulos George, Rice Treva, Rao D C, Bouchard Claude

机构信息

Human Genomics Laboratory, Pennington Biomedical Research Center, Louisiana State University System, Baton Rouge, LA 70808-4124, USA.

出版信息

Circ Cardiovasc Genet. 2010 Jun;3(3):294-9. doi: 10.1161/CIRCGENETICS.109.925644. Epub 2010 Apr 20.

Abstract

BACKGROUND

A genome-wide linkage scan identified a quantitative trait locus for exercise training-induced changes in submaximal exercise (50 W) heart rate (DeltaHR50) on chromosome 2q33.3-q34 in the HERITAGE Family Study (n=472).

METHODS AND RESULTS

To fine-map the region, 1450 tag SNPs were genotyped between 205 and 215 Mb on chromosome 2. The strongest evidence of association with DeltaHR50 was observed with 2 single-nucleotide polymorphisms (SNPs) located in the 5' region of the cAMP-responsive element-binding protein 1 (CREB1) gene (rs2253206: P=1.6x10(-5) and rs2360969: P=4.3x10(-5)). The associations remained significant (P=0.01 and P=0.023, respectively) after accounting for multiple testing. Regression modeling of the 39 most significant SNPs in the single-SNP analysis identified 9 SNPs that collectively explained 20% of the DeltaHR50 variance. CREB1 SNP rs2253206 had the strongest effect (5.45% of variance), followed by SNPs in the FASTKD2 (3.1%), MAP2 (2.6%), SPAG16 (2.1%), ERBB4 (3 SNPs approximately 1.4% each), IKZF2 (1.4%), and PARD3B (1.0%) loci. In conditional linkage analysis, 6 SNPs from the final regression model (CREB1, FASTKD2, MAP2, ERBB4, IKZF2, and PARD3B) accounted for the original linkage signal: The log of the odds score dropped from 2.10 to 0.41 after adjusting for all 6 SNPs. Functional studies revealed that the common allele of rs2253206 exhibits significantly (P<0.05) lower promoter activity than the minor allele.

CONCLUSIONS

Our data suggest that functional DNA sequence variation in the CREB1 locus is strongly associated with DeltaHR50 and explains a considerable proportion of the quantitative trait locus variance. However, at least 5 additional SNPs seem to be required to fully account for the original linkage signal.

摘要

背景

在遗产家族研究(n = 472)中,全基因组连锁扫描在2号染色体2q33.3 - q34区域鉴定出一个与运动训练引起的次极量运动(50 W)心率变化(DeltaHR50)相关的数量性状位点。

方法与结果

为了精细定位该区域,在2号染色体上205至215 Mb之间对1450个标签单核苷酸多态性(SNP)进行了基因分型。在环磷酸腺苷反应元件结合蛋白1(CREB1)基因5'区域的2个单核苷酸多态性(SNP)(rs2253206:P = 1.6×10⁻⁵和rs2360969:P = 4.3×10⁻⁵)观察到与DeltaHR50关联的最强证据。在考虑多重检验后,这些关联仍然显著(分别为P = 0.01和P = 0.023)。单SNP分析中39个最显著SNP的回归模型确定了9个SNP,它们共同解释了DeltaHR50变异的20%。CREB1 SNP rs2253206的效应最强(变异的5.45%),其次是FASTKD2(3.1%)、MAP2(2.6%)、SPAG16(2.1%)、ERBB4(3个SNP,每个约1.4%)、IKZF2(1.4%)和PARD3B(1.0%)位点中的SNP。在条件连锁分析中,最终回归模型中的6个SNP(CREB1、FASTKD2、MAP2、ERBB4、IKZF2和PARD3B)解释了原始连锁信号:在对所有6个SNP进行校正后,优势对数得分从2.10降至0.41。功能研究表明,rs2253206的常见等位基因表现出比次要等位基因显著更低(P < 0.05)的启动子活性。

结论

我们的数据表明,CREB1基因座中的功能性DNA序列变异与DeltaHR50密切相关,并解释了相当比例的数量性状位点变异。然而,似乎至少还需要5个额外的SNP才能完全解释原始连锁信号。

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