Association between G-protein β3 subunit gene and isolated systolic blood pressure elevation of greater than 130 mmHg: A large-scale cross-sectional study in the Japanese population

AIM To investigate whether GNB3 C825 T single nucleotide polymorphism(SNP) contributes to systolic blood pressure(SBP) ≥ 130 mmH g in a large-scale cross-sectional study among the Japanese population with diastolic blood pressure(DBP) < 85 mmH g. METHODS We analyzed 11008 Japanese subjects, including 2797 cases(SBP ≥ 130 and DBP < 85 mmH g) who were not taking anti-hypertensive medication and 8211 controls(SBP < 130 and DBP < 85 mmH g), all of whom enrolled in the genome banking project of the 21 st Century COE(Center of Excellence) Program at Jichi Medical University. Subjects were divided into four groups according to gender(male and female) and age(≤ 49 years and ≥ 50 years). GNB3 gene polymorphism was determined using the TaqM an probe method. We compared the frequencies of alleles and genotypes between cases and controls by chi-squared test. The strength of the associations was estimated by odds ratios(ORs) and 95%CI by using logistic regression analysis. The ORs were adjusted for age and body mass index. RESULTS Allele and genotype distributions significantly differed between cases and controls only in males aged ≤ 49 years. Compared to the CC genotype, a significant OR was obtained in the TT genotype among males aged ≤ 49 years.CONCLUSION This study indicates that the TT genotype of the GNB3 C825 T SNP may contribute to SBP elevation of greater than 130 mmH g compared to the CC genotype in Japanese males aged ≤ 49 years.

G-protein beta 3 subunit polymorphisms and essential hypertension： a case-control association study in northern Han Chinese

Objective To explore the association between the three polymorphisms [ C825T, C1429T and G（-350）A] of the gene encoding the G protein beta 3 subunit （GNB3） and hypertension by performing a case-control study in the northern Han Chinese population. Methods We recnaited 731 hypertensive patients and 673 control subjects （the calculated power value was 〉 0.8）. Genotyping was performed to identify C825T, C1429T and G（-350）A polymorphisms using the TaqMan assay. Comparisons of allelic and genotypic frequencies between cases and controls were made by using the chi-square test. Logistic regression analyses were performed to investigate the relationships between the three polymorphisms of GNB3 gene under different genetic models （additive, dominant and recessive models）. Results The genotype dis- tribution and allele frequencies of C825T, C1429T and G（-350）A polymorphisms did not differ significantly between hypertensive patients and control subjects, either when the full sample was assessed, or when the sample was stratified by gender. No significant association was observed between C825T, C 1429T and G（-350）A polymorphisms and the risk of essential hypertension in any genetic model. Linkage dis- equilibrium was only detected between C825T and C 1429T polymorphisms. Haplotype analyses observed that none of the three estimated haplotypes significantly increased the risk of hypertension. Conclusions Our study suggested that the GNB3 gene polymorphisms [C825T, C 1429T and G（-350）A] were not significantly associated with essential hypertension in northern Han Chinese population.

Gene Cloning and Expression Analysis of G Protein αq Subunit from Helicoverpa assulta (Guenée)

The cDNA encoding the G protein αq subunit was isolated from the antennae of Helicoverpa assulta （Guen6e） by reverse transcription polymerase chain reaction （RT-PCR） and named as HassGαq. Sequencing analysis showed that the fulllength of HassGαq open reading frame （ORF） is 1 062 bp, 353 amino acid residues are encoded. The predicted molecular weights （MW） and isoelectric point （PI） are 41.5 kD and 5.15, respectively. HassGαq gene was then constructed into expression vector pGEX-4T-2 for over expression in prokaryotic cells. The SDS-PAGE and Western blot analysis showed that induced by Isopropyl-β-D-Thiogalactoside （IPTG）, the GST-HassGαq fusion protein is expressed in Escherichia coil BL21, and its MW was found to be about 66 kD nearly equal to the predicted. In addition, RT-PCR analysis showed that the expressions of HassGαq are not tissue specific.

Gene Cloning and Tissue-Specific Expression of G Protein β Subunit in Microplitis mediator (Hymenoptera: Braconidae)

A gene encoding a novel G protein β subunit of β1 subclass, GβMmed was isolated from Microplitis mediator （Hymenoptera： Braconidae）. The full-length sequence of GβMmed is 1 119 bp, the cDNA contains a 1 023 bp open reading frame that encodes a protein with 340 amino acids, and the predicted molecular weight of GβMmed is 37.23 kDa and isoelectric point is 5.86. By the quantitative real-time RT-PCR method, the tissue-specific expression and quantitative changes in the developmental expression profile of GβMmed were detected. It was found that GβMmed was abundantly expressed in M. mediator antennae, head （without antennae）, thorax, abdomen, legs and the wings, and especially at high levels in abdomen. In antennae, expression varied through 1st day before emergence to 5-d-old adults, and had equal expression levels detected in females and males in total. In head, GβMmed expresses while initially high in females, and have another peaked in stage 4 and 1st day, in males showed a peak of GβMmed expression prior to emergence and relatively low levels after emergence. In female abdomen GβMmed expression levels have two peaks in stage 1 and the 5th d, but just have one peak in male abdomen in stage 1. In all other tissues expression was low and stable.

褐飞虱G蛋白β亚基基因的功能分析

【目的】本研究旨在鉴定褐飞虱Nilaparvata lugens G蛋白β亚基基因(NlGβ)并分析其功能,以期为基于RNAi技术防治褐飞虱提供潜在的新靶标基因。【方法】利用PCR克隆并验证褐飞虱NlGβ的编码序列(coding sequence,CDS)并进行生物信息学分析;基于褐飞虱不同发育阶段(卵、1-5龄若虫和雌雄成虫)和成虫不同组织(头、足、肠道、表皮、脂肪体、雌性生殖系统和雄性生殖系统)转录组表达谱分析NlGβ的时空表达模式;通过对2和5龄褐飞虱若虫进行显微注射dsRNA沉默NlGβ,观测个体和雌性生殖系统表型,统计存活率、单雌产卵量和卵孵化率,利用透射电子显微镜技术观察侧输卵管膨大区。【结果】褐飞虱NlGβ(GenBank登录号:XP_022200908.1)的CDS长948 bp,NlGβ蛋白包含7个WD40结构域和4个WD_REPEATS_1基序,是一个较为保守的蛋白,除了直翅目昆虫外,来源于其他昆虫目中的NlGβ同源蛋白能很好地聚集在同一簇进化分支上。NlGβ的表达量在1-3龄若虫期呈现周期性变化,在5龄雌若虫和雌成虫中的表达量高于5龄雄若虫和雄成虫中的;NlGβ在成虫不同组织中都表达,但在脂肪体中表达量最高,在雌性生殖系统中的表达量高于雄性生殖系统中的。沉默褐飞虱2龄若虫NlGβ,出现蜕皮困难的现象,导致存活率较ds GFP对照组显著降低;沉默褐飞虱5龄若虫NlGβ,雌成虫腹部异常膨大,卵巢发育畸形,单雌产卵量较对照组显著下降,卵无法孵化,侧输卵管膨大区内分泌物增加,上皮细胞发生降解。【结论】NlGβ与褐飞虱的生长发育和雌虫的繁殖密切相关。

G蛋白β2亚基对结直肠癌细胞转移能力的影响

目的探讨G蛋白β2亚基(GNB2)对结直肠癌细胞体外迁移和体内转移能力的影响及机制。方法将对数生长期人胚肾细胞293FT随机分为对照组和shGNB2组,对照组293FT细胞转染PSPAX2、PMD2G、Control质粒,shGNB2组293FT细胞转染PSPAX2、PMD2G、shGNB2质粒,分别收集病毒上清液。将对数生长期人结直肠癌细胞HCT116、RKO按随机数字表法分为对照组和shGNB2组,应用293FT细胞对照组病毒上清液转染对照组HCT116和RKO细胞,应用293FT细胞shGNB2组病毒上清液转染shGNB2组HCT116和RKO细胞,应用实时荧光定量聚合酶链反应法检测对照组和shGNB2组HCT116、RKO细胞中GNB2 mRNA的表达,Western blot法检测对照组和shGNB2组HCT116、RKO细胞中GNB2、波形蛋白(Vimentin)、神经钙黏蛋白(N-cadherin)和E-钙黏蛋白(E-cadherin)的表达,划痕愈合实验检测对照组和shGNB2组HCT116、RKO细胞划痕愈合率,Transwell小室实验检测对照组和shGNB2组HCT116、RKO细胞迁移细胞数。分别取对照组和shGNB2组HCT116细胞2×106个注射于裸鼠皮下,3周后取出皮下肿瘤,剪成1 mm 3大小的组织块。按随机数字表法将8只4~5周龄雌性裸鼠分为对照组和shGNB2组,每组4只;将对照组HCT116细胞皮下瘤组织块接种于对照组裸鼠回盲部肠浆膜处,shGNB2组HCT116细胞皮下瘤组织块接种于shGNB2组裸鼠回盲部肠浆膜处;记录裸鼠死亡时间,取出肝脏,观察肝脏肿瘤转移数。结果shGNB2组HCT116、RKO细胞中GNB2 mRNA和蛋白相对表达量显著低于对照组(P<0.01)。培养48 h时,shGNB2组HCT116、RKO细胞划痕愈合率显著低于对照组(P<0.01),shGNB2组HCT116、RKO细胞迁移数显著少于对照组(P<0.01)。shGNB2组裸鼠肝内转移瘤数显著少于对照组(P<0.05)。shGNB2组HCT116、RKO细胞中Vimentin、N-cadherin蛋白相对表达量显著低于对照组,E-cadherin蛋白相对表达量显著高于对照组(P<0.01)。结论干扰GNB2表达可有效抑制结直肠癌细胞的转移能力,其机制可能是GNB2通过调控上皮间质转化过程来参与结直肠癌细胞的转移。

Long non-coding RNA CDKN2B-AS1 promotes hepatocellular carcinoma progression via E2F transcription factor 1/G protein subunit alpha Z axis

BACKGROUND A series of long non-coding RNAs(lncRNAs)have been reported to play a crucial role in cancer biology.Some previous studies report that lncRNA CDKN2B-AS1 is involved in some human malignancies.However,its role in hepatocellular carcinoma(HCC)has not been fully deciphered.AIM To decipher the role of CDKN2B-AS1 in the progression of HCC.METHODS CDKN2B-AS1 expression in HCC was detected by quantitative real-time polymerase chain reaction.The malignant phenotypes of Li-7 and SNU-182 cells were detected by the CCK-8 method,EdU method,and flow cytometry,respectively.RNA immunoprecipitation was executed to confirm the interaction between CDKN2B-AS1 and E2F transcription factor 1(E2F1).Luciferase reporter assay and chromatin immunoprecipitation were performed to verify the binding of E2F1 to the promoter of G protein subunit alpha Z(GNAZ).E2F1 and GNAZ were detected by western blot in HCC cells.RESULTS In HCC tissues,CDKN2B-AS1 was upregulated.Depletion of CDKN2B-AS1 inhibited the proliferation of HCC cells,and the depletion of CDKN2B-AS1 also induced cell cycle arrest and apoptosis.CDKN2B-AS1 could interact with E2F1.Depletion of CDKN2B-AS1 inhibited the binding of E2F1 to the GNAZ promoter region.Overexpression of E2F1 reversed the biological effects of depletion of CDKN2B-AS1 on the malignant behaviors of HCC cells.CONCLUSION CDKN2B-AS1 recruits E2F1 to facilitate GNAZ transcription to promote HCC progression.

Frequency of C825T G protein β3 subunit gene polymorphism and its association with obesity in the Kyrgyz population

Objective:To examine the frequency of C825T G protein β3 subunit gene polymorphism and its association with obesity of ethnic Kyrgyz.Methods:The study enrolled 210 people,89 patients(35 females,54 males)with obesity(BMI≥30 kg/m2)and 121 practically healthy patients(38 females,83 males)with normal body weight and no signs of type 2 diabetes(group of control),who were not observed before by a cardiologist.The blood pressure,anthropometry,glucose and lipid profile were examined among all subjects.Genomic DNA was extracted from peripheral blood cells.G proteinβ3 subunit C825T polymorphism was determined by polymerase chain reaction(PCR).Results:TT and CT genotypes carriers were grouped together in one group because the TT genotype was rare.CT+TT genotype frequency in the group with obesity made 0.72 and was significantly higher than that in the control group-0.52(χ2-8.44;P=0.004;odds ratio-2.55;95%CI 1.31-4.23).The statistical analysis revealed that hypertension(45%vs.31.3%,P=0.049)and obesity(51.2%vs.30%,P<0.01)occurred significantly more often in CT+TT genotype carriers than in the CC homozygotes.The results of the multivariate logistic regression analysis showed that the presence of 825T allele(exp β-2.89;95%CI 1.25-6.7;P=0.013),along with the occasional consumption of vegetables(exp β-3.47;95%CI 1.52-7.94;P=0.003)was the significant risk factor for obesity,regardless of gender,age and level of physical activity.In the construction of the similar regression model for hypertension,the statistically significant role of 825T allele was lost after adjustment for obesity as an independent variable.Conclusion:G protein β3 subunit gene C825T allele in the Kyrgyz ethnic group has an association with obesity.

MFG-E8和GNA14在子宫内膜异位症相关性卵巢癌中的表达及其临床意义

目的探讨乳脂球表皮生长因子8(MFG-E8)和G蛋白亚基α-14(GNA14)在子宫内膜异位症相关性卵巢癌(EAOC)中的表达及其临床意义。方法选取2015年5月—2017年5月华北医疗健康集团峰峰总医院EAOC患者51例(EAOC组)、非典型子宫内膜异位症(AEM)患者63例(AEM组)、卵巢型子宫内膜异位症(EMT)患者82例(EMT组)。收集所有患者的临床资料,并检测病变组织中MFG-E8、GNA14表达。对EAOC患者随访5年。采用Kaplan-Meier生存曲线分析EAOC患者的生存情况。采用多因素Cox回归分析评估EAOC患者死亡的危险因素。结果EAOC组MFG-E8阳性率为82.35%、GNA14阳性率为70.59%,均显著高于AEM组(41.27%、44.44%)和EMT组(25.61%、23.17%)(P<0.001)。MFG-E8高表达组和低表达组肿瘤直径、肿瘤级别、国际妇产科联合会(FIGO)分期、淋巴转移情况差异均有统计学意义(P<0.05)。GNA14高表达组和低表达组淋巴转移情况差异有统计学意义(P=0.009)。Kaplan-Meier生存曲线分析结果显示,MFG-E8高表达组和GNA14高表达组无进展生存期分别短于MFG-E8低表达组和GNA14低表达组(P<0.05)。多因素Cox回归分析结果显示,FIGO分期Ⅱ期、淋巴转移、MFG-E8高表达、GNA14高表达是EAOC患者死亡的独立危险因素[风险比(HR)值分别为2.337、2.519、3.133、3.080,95%可信区间(CI)分别为1.258~4.342、1.332~4.764、1.381~7.108、1.318~7.197,P<0.01]。结论MFG-E8、GNA14在EAOC患者癌组织中呈高表达,且与患者预后不良密切相关,或可作为EAOC患者的预后评估指标。

G-protein β subunit AGB1 positively regulates salt stress tolerance in Arabidopsis

The heterotrimeric GTP-binding proteins（G-proteins） in eukaryotes consisted of α, β and γ subunits and are important in molecular signaling by interacting with G-protein-coupled receptors（GPCR）, on which to transduce signaling into the cytoplast through appropriate downstream effectors. However, downstream effectors regulated by the G-proteins in plants are currently not well defined. In this study, the transcripts of AGB1, a G protein β subunit gene in Arabidopsis were found to be down-regulated by cold and heat, but up-regulated by high salt stress treatment. AGB1 mutant（agb1-2） was more sensitive to high salt stress than wild-type（WT）. Compared with WT, the cotyledon greening rates, fresh weight, root length, seedling germination rates and survival rates decreased more rapidly in agb1-2 along with increasing concentrations of Na Cl in normal（MS） medium. Physiological characteristic analysis showed that compared to WT, the contents of chlorophyll, relative proline accumulation and peroxidase（POD） were reduced, whereas the malonaldehyde（MDA） content and concentration ratio of Na＋/K＋ were increased in agb1-2 under salt stress condition. Further studies on the expression of several stress inducible genes associated with above physiological processes were investigated, and the results revealed that the expressions of genes related to proline biosynthesis, oxidative stress response, Na＋ homeostasis, stress- and ABAresponses were lower in agb1-2 than in WT, suggesting that those genes are possible downstream genes of AGB1 and that their changed expression plays an important role in determining phenotypic and physiologic traits in agb1-2. Taken together, these findings indicate that AGB1 positively regulates salt tolerance in Arabidopsis through its modulation of genes transcription related to proline biosynthesis, oxidative stress, ion homeostasis, stress- and ABA-responses.

非染色体结构维护凝集素Ⅰ复合物亚基G通过Akt信号通路促进卵巢癌细胞的增殖、迁移和侵袭

目的探讨非染色体结构维护凝集素Ⅰ复合物亚基G(NCAPG)调控卵巢癌细胞的增殖、迁移和侵袭的机制。方法生物信息学GEPIA数据库分析NCAPG在卵巢癌组织中的差异表达。Western blotting检测正常卵巢上皮细胞IOSE80、卵巢癌A2780和SKOV3细胞中NCAPG的蛋白表达。NCAPG siRNA沉默实验分为空白组、对照组、siNCAPG-1组和siNCAPG-2组。NCAPG过表达实验分为空白组、对照组、NCAPG组、NCAPG+MK2206组和MK2206组。MTT实验检测细胞增殖活性;细胞划痕实验和Transwell实验评估细胞的迁移和侵袭能力;Western blotting检测细胞的磷酸化Akt(p-Akt)、总Akt(t-Akt)、增殖细胞核抗原(PCNA)、基质金属蛋白酶9(MMP-9)、波形蛋白(vimentin)、N-钙黏蛋白(N-cadherin)和E-钙黏蛋白(E-cadherin)的表达水平。结果NCAPG在卵巢癌组织和卵巢癌细胞中高表达。沉默NCAPG可明显抑制卵巢癌SKOV3细胞的增殖、迁移和侵袭,p-Akt、PCNA、MMP-9、vimentin和N-cadherin表达减少,E-cadherin表达增多。过表达NCAPG质粒可促进卵巢癌A2780细胞增殖、迁移和侵袭,p-Akt、PCNA、MMP-9、vimentin和N-cadherin表达增多,E-cadherin表达降低。Akt抑制剂MK2206可明显抑制NCAPG的上述作用。结论NCAPG激活Akt信号通路,调控PCNA、MMP-9和上皮细胞-间充质转化(EMT)相关蛋白的表达,促进卵巢癌细胞的增殖、迁移和侵袭。

香蕉枯萎病菌fga1基因的克隆与序列分析

为了解fga1基因在尖孢镰刀菌古巴专化型侵染香蕉过程中的作用,及其与尖孢镰刀菌古巴专化型生理小种1号和生理小种4号之间的致病力差异的关系,采用PCR和RT-PCR方法扩增了2个生理小种的fga1基因,并对扩增产物进行了测序及相似序列搜索和比对,还对基因编码的蛋白进行了氨基酸序列比对和功能分析。研究结果表明2个生理小种fga1基因开放阅读框均为1062bp,编码353个氨基酸,基因同源性为99.5%,氨基酸序列相同。推测fga1基因可能与香蕉枯萎病菌自身繁殖和附着胞的形成有关。从fga1基因序列及其编码蛋白的氨基酸序列看,2个生理小种致病力的差异与fga1基因并无明显对应关系,这为进一步研究fga1基因功能奠定了基础。

桔小实蝇V-ATPaseG亚基基因的克隆及组织表达特异性分析

空泡型ATP酶(vacuolar-type H+-ATPase,V-ATPase)作为质子泵几乎在所有的真核生物细胞中发挥重要作用。本研究利用RT-PCR和RACE技术获得了桔小实蝇Bactrocera dorsalis(Hendel)V-ATPase G亚基序列全长,命名为BdorATPG。测序结果表明,BdorATPG阅读框全长354bp,编码117个氨基酸。氨基酸序列比对表明,BdorATPG的N端序列与其他物种的ATPG亚基对应区域具有较高的序列一致性。BdorATPG与拟暗果蝇Drosophila pseudoobscura ATPG亚基的氨基酸序列一致性最高,为88.9%。三维结构模建结果表明,BdorATPG N端(第1～59位氨基酸)序列为α-螺旋结构,亲水性和疏水性氨基酸在螺旋两侧呈对称分布。BdorATPG在不同组织中的荧光定量PCR分析表明,BdorATPG在各组织中都有表达,其中在触角中的表达量最高;在雄虫生殖节中的表达量是雌虫中的6.04倍。结果提示BdorATPG可能在雄虫生殖生理过程中发挥重要作用。

G蛋白β3亚基基因C825T多态性与抑郁症及SSRI和SNRI类抗抑郁药疗效关系的探讨

目的:研究G蛋白β3亚基基因C825T多态性与抑郁症及治疗是否存在相关性。方法:采用聚合酶链式反应-限制性片段长度多态性分析（PCR-RFLP）技术对140例抑郁症患者和100例健康志愿者进行基因型分析;用HAMD评定抑郁症的疗效。结果:抑郁症Gβ3基因基因型频率（CC20.7％,CT31.4％,TT47.9％）、等位基因频率（C3.64％,T63.6％）;与正常对照组基因频率（CC27.0％,CT51.0％,TT22.0％）、等位基因频率（C52.5％,T47.5％）比较具有显著性差异;不同基因型抑郁症患者经4周SSRI、SNRI类抗抑郁药治疗后,HAMD总分均显著下降,减分率有显著差异。结论:本研究提示在中国人群中G蛋白β3亚基基因C825T多态性与抑郁症及抗抑郁药疗效有关。

MiAsg分子克隆及与南方根结线虫病害的关系

根结线虫(Meloidogyne spp.)是一种世界性的植物病害。在前期研究中,通过利用生物信息学方法在线虫全基因组中预测了一些功能基因。本研究以预测到的线粒体ATP合成酶g亚基基因(Asg)序列设计特异引物克隆了南方根结线虫(M.incognita)的Asg基因(MiAsg),对其序列进行了特征分析后,利用病毒诱导的基因沉默(VIGS)技术,将其导入番茄植株,然后接种M.incognita,研究MiAsg基因与根结线虫病害的关系。结果表明,克隆到的MiAsg基因与预测到的MiAsg基因相似性高达100%。接种M.incognita 60 d后,MiAsg基因沉默的番茄植株根结数分别比空载体对照减少了59.6%,比清水对照降低了59.5%。结果表明,MiAsg基因沉默对根结线虫病害具有很好的防控效果,也说明MiAsg基因可能参与线虫的致病性。

IgG抗体及其亚类在超敏反应中的作用

IgE抗体与超敏反应尤其是速发型超敏反应的关系已得到公认,IgG抗体在超敏反应中的作用至今尚未阐明。IgG抗体分为IgG1,IgG2,IgG3和IgG44个亚类。针对不同的过敏原、过敏阶段及患者过敏体质IgG抗体亚类对超敏反应的发生可发挥介导或抑制作用。随着人们对IgG抗体及其亚类认识的逐步深入,IgG抗体及其亚类在超敏反应中的作用、在诊断和治疗中的应用将逐步得到阐明。

在中国北方汉族人群中血管紧张素转换酶基因I/D多态与G蛋白beta3亚基基因C825T多态对原发性高血压的联合作用(英文)

原发性高血压是一种复杂的多基因疾病,被认为是多个变异了的基因遗传交互以及环境因素共同作用的结果.证据表明,血管紧张素转换酶基因和G蛋白beta3亚基基因各自都是重要的原发性高血压的易感基因,并且可能存在共同的通路来导致高血压疾病的发展.为了探索这两个基因在中国北方汉族人群中是否对高血压有影响,挑选血管紧张素转换酶基因I/D多态与G蛋白beta3亚基基因C825T多态,在一个包含502个高血压病例和490个健康对照的样本中做了关联研究.连锁不平衡分析揭示,仅仅在男性中有显著性的非随机性分布,表明血管紧张素转换酶基因与G蛋白beta3亚基基因倾向在男性中造成高血压.调整了的单位点的多变量逐步回归分析展示,在男性显性模型中DD/ID对Ⅱ的比值比达到显著性水平(OR1.57;95%CI,1.09～2.27;P=0.016).在对性别进行分层后的联合分析中,在男性中经过调整后的比值比具有弱显著性水平:在血管紧张素转换酶基因的DD基因型中,TT对CC的比值比是0.11;95%CI,0.01～0.99;P=0.049;在G蛋白beta3亚基基因的CC+CT基因型中,DD/ID对Ⅱ的比值比是1.52;95%CI,1.01～2.29;P=0.047.结果暗示,血管紧张素转换酶基因或附近的某个基因是具有男性性别倾向的高血压易感侯选基因,同时,在血管紧张素转换酶基因基因的D等位基因和G蛋白beta3亚基基因的825C等位基因之间,可能存在具有上位效应的基因-基因相互作用.

G蛋白β3亚单位基因C825T多态性与蒙古族原发性高血压的相关性研究

目的探讨G蛋白β3亚单位基因C825T多态性与蒙古族人群原发性高血压患者之间的关系。方法采用Sequenom系统检测分析方法检测124例健康人和143例高血压患者的G蛋白β3亚单位基因C825T多态性。结果（1）蒙古族人群GNB3基因C825T位点CC、CT、TT基因型频率在高血压组和正常血压组分别为0．48、0．41、0．11和0．43、0．47、0．10，差异无显著性（χ^2=0．162，P=0．688；OR：1．176，95％CI 0．533～2．592）；C、T等位基因频率在高血压组和对照组分别为0．69、0．31和0．67、0．33差异无显著性（χ^2=0．094，P=0．759；OR：0．945，95％CI0．657—1．358）。（2）蒙古族人群GNB3基因C825T位点CC、CT、TT基因型频率在单纯收缩压增高组和正常血压组分别为0．57、0．35、0．08和0，43、0．47、0．10．差异无显著性（χ^2=0．733．P=0．392；OR：1．957，95％CI0．623—6．143）；C、T等位基因频率在单纯高血压组和对照组分别为0．74、0．26和0．67、0．33，差异无显著性（χ^2=2．133，P=0．144；OR：0．697，95％CI0．428—1．133）。结论G蛋白β3亚单位基因C825T位点与蒙古族人群原发性高血压的发生可能无关，不是蒙古族人群原发性高血压的遗传标志．

家蚕G蛋白γ1亚基(BmGγ1)的克隆及其谷胱甘肽硫转移酶融合蛋白的表达与纯化

异三元G蛋白是真核细胞感知外界信号后将信号传递到胞内的重要分子,参与生物体广泛的信号转导。为了研究家蚕体内G蛋白的生理功能及其作用机制,运用生物信息学方法预测了家蚕G蛋白γ1亚基(Gγ1)的序列,设计引物验证预测序列后,克隆了家蚕Gγ1的序列,再通过酶切克隆至表达载体pET-41b(+)后,导入E.coliBL21宿主菌中,经异丙基β-D-硫代半乳糖苷(IPTG)诱导表达重组谷胱甘肽硫转移酶(glutathione s-transferase,GST)融合蛋白,并亲和层析纯化表达产物。家蚕Gγ1重组GST融合蛋白经SDS-PAGE电泳和Western blot分析,在分子质量约36 kD处出现特异性蛋白条带,重组蛋白经GST亲和层析柱纯化后,得到了高纯度的融合蛋白,说明已经成功克隆到家蚕Gγ1基因,并在E.coliBL21中高效表达。

G蛋白β3亚单位基因C825T多态性对氨氯地平降压效果的影响

目的探讨G蛋白β3亚单位基因C825T多态性与氨氯地平降压疗效的关系。方法采用多聚酶链式反应结合限制性内切酶片段长度多态分析方法,检测147例健康人和321例原发性高血压患者的G蛋白β3亚单位C825T多态性,其中48例高血压患者口服氨氯地平4周。结果1)高血压组G蛋白β3亚单位C825T多态性中基因型频率(CC 28.7%、CT52.0%、TT 19.3%)、等位基因频率(C 54.7%、T 45.3%)与正常对照组基因型频率(CC 27.2%、CT 46.9%、TT 25.9%)、等位基因频率(C 50.7%、T 49.3%)比较差异无统计学意义;2)CC基因型的收缩压降低值〔(4.93±2.26)kPa(37.00±16.97)mmHg〕明显高于CT+TT基因型〔(2.99±1.41)kPa(22.40±10.60)mmHg〕(P<0.05)。结论G蛋白β3亚单位基因C825T多态性与氨氯地平的降压疗效相关,而与原发性高血压无关。