梅花鹿MSRB3基因多态性及其与茸重性状的关联分析

【目的】本研究旨在探索梅花鹿甲硫氨酸亚砜还原酶B3(methionine sulfoxide reductase B3,MSRB3)基因多态性及其与茸重性状的关联性。【方法】选取高、低产茸量的梅花鹿各8只,应用DNA直接测序法检测基因变异位点。采用MassARRAY SNP分型技术对314头24月龄梅花鹿MSRB 3基因进行基因分型,并结合梅花鹿茸重性状数据进行了关联分析和单倍型分析。【结果】在梅花鹿MSRB 3基因中共发现6个SNPs位点,其中2个SNPs位点位于外显子区域,且突变均未引起氨基酸改变,属于同义突变,其余4个SNPs位点均存在于内含子区域。分型结果显示4个样本未分型成功,其余310个样本进行后续分析。各位点观测杂合度和期望杂合度基本一致,g.44455582 T>C、g.44455759 C>T、g.44414424 T>C、g.44350306 T>C及g.44340836 G>A等5个位点的杂合度较高,均属于中度多态(0.25<PIC<0.5),g.44340734 G>C位点杂合度较低,属于低度多态(PIC<0.25)。卡方检验结果表明,g.44455759 C>T位点偏离Hardy-Weinberg平衡状态(P<0.05),其他5个位点均处于Hardy-Weinberg平衡状态(P>0.05)。对6个SNPs位点的不同基因型与梅花鹿茸重的关联分析结果表明,g.44455582 T>C位点的TT基因型个体茸重极显著高于CC和TC基因型(P<0.01)。单倍型分析结果显示,g.44340734 G>C和g.44350306 T>C、g.44455582 T>C和g.44455759 C>T位点存在强连锁,各产生3种单倍型,在Block 2区块中单倍型TC茸重显著高于单倍型CT(P<0.05)。【结论】MSRB 3基因与梅花鹿茸重性状密切相关,g.44455582 T>C位点和单倍型TC可作为筛选高产梅花鹿的分子标记。

MSRB3作为致癌新基因可独立预测宫颈癌患者的不良预后

目的:基于癌症基因组图谱(TCGA)数据库和GSEA富集分析,探讨甲硫氨酸亚砜还原酶B3(MSRB3)在宫颈癌中的作用及相关机制。方法:从TCGA数据库中下载宫颈癌基因数据及临床特征数据。采用单变量和多变量Cox生存分析筛查预后差异表达基因MSRB3。使用Kolmogorov-Smirnov检验和Logistic回归分析评估MSRB3与临床病理特征间的关系,Kaplan-Meier用于评估MSRB3与生存率间的相关性。采用GSEA功能富集分析软件分析MSRB3参与宫颈癌发生发展的信号通路及相关生物学功能。结果:相对于正常对照组,MSRB3在宫颈癌组织中低表达。Kaplan-Meier生存分析发现,MSRB3高表达的患者预后较差(P=0.002)。MSRB3表达的增加与宫颈癌的等级分类(Ⅰ、Ⅱ、Ⅲ和Ⅳ的OR=7.34)和年龄(OR=2.54,P<0.05)有关。单变量Cox分析(P=0.040,HR=1.05)和多变量分析(P=0.028,HR=1.07)显示MSRB3与总生存期显著相关。GSEA-KEGG分析证实MSRB3主要富集于MAPK、TGF-β和WNT信号通路;GSEA-GO分析表明,MSRB3主要参与的生物学功能有血管生成、血管形态发生等。结论:MSRB3作为致癌新基因可独立预测宫颈癌患者的不良预后。此外,MSRB3可能主要通过参与MAPK/TGF-β信号途径来发挥其生物学功能,从而影响宫颈癌的发生发展。

Porcine methionine sulfoxide reductase B3:molecular cloning,tissue-specific expression profiles,and polymorphisms associated with ear size in Sus scrofa

Background： In Sus scrofa, methionine sulfoxide reductase B3（MSRB3） is a crucial candidate gene for ear size, and an important conformational trait of pig breeds. However, challenges in MSRB3 c DNA amplification have prevented further identification of MSRB3 allelic variants influencing pig ear size.Results： We cloned a full-length c DNA sequence of porcine MSRB3 by rapid-amplification of c DNA ends. The3,765-bp gene contained a 5＇-untranslated region（UTR）（190 bp）, a coding region（552 bp）, and a 3＇-UTR（3,016 bp） and shared 84 %, 84 %, 87 %, 86 %, and 70 % sequence identities with human, orangutan, mouse, chicken, and zebrafish,respectively. The gene encoded a 183-amino acid protein, which shared 88 %, 91 %, 89 %, 86 %, and 67 % identities with human, orangutan, mouse, chicken, and zebrafish, respectively. Tissue expression analysis using q RT-PCR revealed that MSRB3 was expressed in the heart, liver, lung, kidney, spleen, ear, muscle, fat, lymph, skeletal, and hypothalamic tissues. Three single nucleotide polymorphisms（SNPs） were identified in MSRB3： c.-735 C 〉 T in the 5＇ flanking region,c.2571 T 〉 C in the 3＇-UTR, and a synonymous mutation of c.484 T 〉 C in the coding region. The SNPs c.-735 C 〉 T and c.2571 T 〉 C were significantly associated with ear size in a Large White × Minzhu F2 population other than in Beijing Black pigs. Subsequently, at SNP c.-735 C 〉 T, the m RNA of MSRB3 was significantly higher expressed in ears of individuals with the TT genotype（Minzhu） than those with CC（Large White）.Conclusions： The porcine MSRB3 owned a 3,765-bp full-length c DNA sequence and was detected to express in ear tissue. Two SNPs of this gene were shown to be significantly associated with ear size in a Large White × Minzhu intercross population instead of Beijing Black pig population. What＇s more, the individuals with higher m RNA expression of MSRB3 have larger ear sizes. These results provide useful information for further functional analyses of MSRB3 influencing ear size in pigs.