The preparation and application of N-terminal 57 amino acid protein of the follicle-stimulating hormone receptor as a candidate male contraceptive vaccine

Follicle-stimulating hormone receptor （FSHR）, which is expressed only on Sertoli cells and plays a key role in spermatogenesis, has been paid attention for its potential in male contraception vaccine research and development. This study introduces a method for the preparation and purification of human FSHR 57-amino acid protein （FSHR-57aa） as well as determination of its immunogenicity and antifertility effect. A recombinant pET-28a（＋）-FSHR-57aa plasmid was constructed and expressed in Escherichia coil strain BL21 StarTM （DE3） and the FSHR-57aa protein was separated and collected by cutting the gel and recovering activity by efficient refolding dialysis. The protein was identified by Western blot and high-performance liquid chromatography analysis with a band of nearly 7 kDa and a purity of 97.4%. Male monkeys were immunized with rhFSHR-57aa protein and a gradual rising of specific serum IgG antibody was found which reached a plateau on day 112 （16 weeks） after the first immunization. After mating of one male with three female monkeys, the pregnancy rate of those mated with males immunized against FSHR-57aa was significantly decreased while the serum hormone levels of testosterone and estradiol were not disturbed in the control or the FSHR-57aa groups. By evaluating pathological changes in testicular histology, we found that the blood-testis barrier remained intact, in spite of some small damage to Sertoli cells. In conclusion, our study demonstrates that the rhFSHR-57aa protein might be a feasible male contraceptive which could affect sperm production without disturbing hormone levels.

Cloning and Transcriptional Activity of Follicle-Stimulating Hormone Receptor Promoter in the Jintang Black Goat

[ Objective] To clone follicle-stimulating hormone receptor （FSHR） promoter in the Jintang black goat, study its transcriptional activity, and provide a basis for alternative splicing of FSHR gene. [Method] The total DNA were extracted from the womb of Jintang black goat, and one pair of primers were designed for amplification of FSHR promoter fragments, then the sequences and homology were analyzed. The FSHR promoter fragment was inserted into the pcFSHRB1 expression vector to substitute the CMV promoter and construct the pcFSHRB2 expression vector. The pcFSHRB1 and pcFSHRB2 expression vectors were transformed into HEK293 cells, respectively. Then these cells were collected after 24 and 48 h treatment with 2 mlU/ml follicle-stimulating hormone （FSH）, and the cAMP levels were detected. [Result] The FSHR promoter sequence of Jin- tang black goat had 34.2% homology to that of chicken and 41.6% to that of rat, respectively. The transcription initial site of FSHR was at -576 bp and its upstream sequences contained two TATA-boxes, four CAAT-boxes, one E-box and one Wl-box. After treating for 24 and 48 h, the cAMP levels of pcFSHRB2 were respectively 299.581 3 and 125.528 1 pmol/L; and that of pcFSHRB1 were respectively 120.057 1 and 109.940 7 pmoVL. [Conclusion] The FSHR promoter of Jintang black goat is a typical type 2 eukaryotic promoter, and it is also a strong promoter.

Effects of Antisense Oligodeoxynucleotide to Follicle-stimulating Hormone Receptor on the Cell Proliferation and Apoptosis in Cells Derived from Human Ovarian Mucinous Cystadenocarcinoma in Vitro

The human ovarian mucinous cystadenocarcinoma （hOMC） cells were co-cultured with antisense oligodeoxynucleotide （antisense ODN）, nonsense ODN, and follicle-stimulating hormone （FSH） at different concentrations for the purpose of observing the effects of antisense ODN to FSH receptor （FSHR） on the proliferation and apoptosis of cultured hOMC cells in vitro. The inhibitory rates of growth were measured by using MTT method on the 2nd, 4th, 6th, 8th and 10th days after the interference of antisense ODN, nonsense ODN, and FSH, respectively. The apoptotic rates and the cell cycles were determined by means of flow cytometry, the apoptosis indexes were detected by using TUNEL, and the expression of caspase-3 was measured by using SP immunohistochemistry. Compared with that in the control group, the proliferative activity of hOMC cells was increased obviously in FSH groups （P〈0.05 or P〈0.01）, decreased distinctly in antisense ODN groups （P〈0.05 or P〈0.01）, and unchanged in nonsense ODN groups, respectively. Meanwhile, antisense ODN could significantly antagonize the FSH-promoted cell proliferative activity （P〈0.01）. Compared with those in the control group, the apoptotic rates and the expression of caspase-3 were dramatically increased in the mid- and high-dose antisense ODN groups （P〈0.05 or P〈0.01）, while the number of cells in G1/G0 phase was significantly decreased and that in S phase distinctly increased （P〈0.01）, There was no change in nonsense ODN groups （P〉0.05）, It was suggested that FSH may improve the development of hOMC cells, However, antisense ODN could inhibit proliferative activity and the FSH-promoted proliferative activity in hOMC cells, at the same time, antisense ODN could inhibit hOMC cell growth by inducing apoptosis.

Polymorphism of Follicle-Stimulating Hormone Receptor Gene in Ningxia Tan Sheep

[ Objective] To study the polymorphism of follicle-stimulating hormone receptor （FSHR） gene in Ningxia Tan sheep and thus to provide a theoretical basis for breeding. I Methodl Genotypes of 111 healthy Ningxia Tan sheep were examined by polymerase chain reaction and restriction fragment length polymorphism （PCR-RFLP）. [ResultS] A 306-bp fragment was amplified. The PCR products digested with restriction enzyme Alu I showed polymorphism with three genotypes, L e., GG, CG and CC. The genotypic frequencies of GG, CG and CC were 0.135 1 （ 15 individuals）, 0.666 7 （74 individuals） and 0.198 2 （22 individuals）, respectively. The allele frequencies of G and C were 0.468 5 and 0.531 5, respectively.[ Conclusion] FSHR aene is Dolvmomhic in Ninaxia Tan Sheeo.

The Determination and Evaluation of the Biological Activities for the Commercialization of Recombinant Follicle-Stimulating Hormone in Vitro

Follicle-stimulating hormone (FSH) plays a central role in mammals reproduction, with the actions of FSH mediated by follicle-stimulating hormone receptors (FSHRs) on the surface of target cells. The purposes of this study were to determine and evaluate the biological activities for the commercialization of recombinant follicle-stimulating hormone (rFSH) in vitro through the cellular internalization using cloned 293T-FSHR cell lines as target. Using imaging approaches we have found here that a little fluorescent signal from the surface of the cell transferred to the cytoplasm and accumulated around the nucleus by endocytosis. Compared with the control groups, the commercialization of rFSH have not the significant differences of internalization, but the rFSH have promoted the internalization of the fluorescent, suggested that this detection system might as a protocol for the bioactivity of recombinant therapeutic proteins in vitro.

关元命门序贯针刺激活FSHR/cAMP/PKA通路促进早发性卵巢功能不全模型大鼠颗粒细胞增殖的机制研究

【目的】观察关元命门序贯针刺方案对早发性卵巢功能不全(POI)模型大鼠的治疗作用及机制。【方法】将雌性SD大鼠分为空白组、模型组、蛋白激酶A(PKA)抑制剂(H89)+针刺组、针刺组各12只。除空白组,其他3组大鼠采用雷公藤多苷片灌胃制备POI模型。模型成功建立后,空白组和模型组每日捆绑一次;针刺组大鼠在动情间期取关元穴针刺,在动情前期取命门穴针刺;H89+针刺组按照针刺组针刺方案干预,在每次针刺前30 min内腹腔注射H89。连续干预20 d。各组大鼠分别在干预后第1个动情间期和动情前期取材。酶联免疫吸附分析(ELISA)检测动情间期促卵泡激素(FSH)、雌二醇(E2)水平,Western Blot法检测动情间期促卵泡激素受体(FSHR)、芳香化酶P450(P450arom)蛋白表达,细胞计数试剂盒8(CCK-8)法检测动情间期和动情前期颗粒细胞活性,免疫组织化学法检测动情前期增殖细胞核抗原(PCNA)蛋白表达水平。【结果】(1)与空白组比较,模型组和H89+针刺组血清FSH水平显著升高(P<0.01),E2水平显著降低(P<0.001);H89+针刺组FSH水平与模型组无差异(P>0.05),E2水平低于模型组(P<0.05);针刺组FSH水平低于模型组和H89+针刺组(P<0.05),与空白组无差异(P>0.05),E2水平显著高于模型组和H89+针刺组(P<0.01),仍低于空白组(P<0.05)。(2)模型组和H89+针刺组FSHR、P450arom蛋白表达均低于空白组(P<0.01);H89+针刺组FSHR蛋白表达水平与模型组无差异(P>0.05),P450arom蛋白表达水平低于模型组(P<0.05);针刺组FSHR、P450arom蛋白表达水平均高于模型组和H89+针刺组(P<0.05),但仍低于空白组(P<0.05)。(3)模型组和H89+针刺组GCs活性和PCNA平均光密度值均低于空白组(P<0.05);H89+针刺组GCs活性和PCNA平均光密度值均低于模型组(P<0.05);针刺组的GCs活性和PCNA平均光密度值显著高于模型组和H89+针刺组(P<0.05或P<0.01)。【结论】关元命门序贯针刺方案可通过上调促卵泡激素受体(FSHR)/环磷酸腺苷(cAMP)/蛋白激酶A(PKA)通路FSHR、P450arom蛋白的表达,调控性激素水平,提高GCs活性和促进GCs细胞增殖,从而改善POI。

Fluoride Exposure,Follicle Stimulating Hormone Receptor Gene Polymorphism and Hypothalamus-pituitary-ovarian Axis Hormones in Chinese Women

The effects of fluoride exposure on thefunctions of reproductive and endocrine systemshave attracted widespread attention in academiccircle nowadays. However, it is unclear whether thegene-environment interaction may modify thesecretion and activity of hypothalamus-pituitary-ovarian （HPO） axis hormones. Thus, the aim of thisstudy was to explore the influence of fluorideexposure and follicle stimulating hormone receptor（FSHR） gene polymorphism on reproductivehormones in Chinese women. A cross sectionalstudy was conducted in seven villages of HenanProvince, China during 2010-2011. A total of 679women aged 18-48 years were recruited throughcluster sampling and divided into three groups, i.e.endemic fluorosis group （EFG）, defluoridationproject group （DFPG）, and control group （CG） basedon the local fluoride concentration in drinkingwater. The serum levels of gonadotropin releasinghormone （GnRH）, follicle stimulating hormone（FSH）, luteinizing hormone （LH）, and estradiol （E2）were determined respectively and the FSHRpolymorphism was detected by real time PCR assay.The results provided the preliminary evidenceindicating the gene-environment interaction onHPO axishormones in women.

黄牛FSHR基因的生物信息学分析

利用生物基因组学数据库,对黄牛FSHR基因进行生物信息学分析,以预测FSHR基因编码产物的理化性质、结构与功能,同时构建FSHR同源系统进化树.结果表明:FSHR基因编码产物为疏水性跨膜蛋白,具有明显的信号肽,其切割位点位于17～18位的氨基酸之间,二级结构主要以α-螺旋与无规则卷曲为主,并主要在质膜中发挥生物学作用,跨膜区域分为跨膜域、胞外域和胞内域3个部分.序列分析表明,FSHR编码产物可能具有离子通道、运载体、受体、信号转导和阳离子通道等功能,在离子跨膜与信号传递过程中发挥重要作用,并对黄牛的激素调节有影响.FSHR基因编码产物系统进化树表明,黄牛FSHR与水牛、成都麻羊、绵羊等物种FSHR遗传距离较近,具有高度同源性.

牛FSHR基因第10外显子单核苷酸多态性及其与双胎性状的关系

以秦川牛和荷斯坦奶牛的双胎母牛和单胎母牛为实验材料 ,以牛的FSHR基因的第 10个外显子作为标记牛双胎性状的候选基因 ,用SNP法进行了多态检测 .结果发现 ,在秦川牛的双胎母牛中突变率 6 0 % (6 10 ) ,而在单胎母牛中突变率为 2 0 % (2 10 ) ;在荷斯坦奶牛中 ,双胎母牛突变率为31 2 5 % (5 16 ) ,单胎母牛突变率为 6 6 7% (1 15 ) ;由此可见双胎牛和单胎牛二者之间FSHR基因的第 10个外显子的突变率差异明显 .这表明 ,选择FSHR基因的第 10个外显子有可能作为双胎性状的候选基因 .序列分析发现 ,在FSHR基因的第 15 0 6位碱基发生了突变 (T→C) ,但氨基酸没有发生变化 .

文昌鸡促卵泡素受体(FSHR)基因外显子区域SNPs分析

寻找与鸡繁殖性能相关的遗传标记,为高繁殖力的标记辅助选择提供科学依据。本研究以促卵泡素受体(FSHR)基因作为影响鸡繁殖性状的候选基因,采用PCR-SSCP技术结合测序对FSHR基因部分包括所有外显子区域进行单核苷酸多态性检测和分析。结果发现,在区域2、区域4、区域6、区域9共4个区域存在SNPs位点。exon4编码区43bp处T→C突变,但没有导致翻译后氨基酸序列的改变,在exon2中编码区5′端—49bp处的C→T突变;exon6编码区3′端+12bp处的A→G突变;exon8编码区3′端+38bp处的G→T突变。促卵泡素受体(FSHR)是促卵泡素(FSH)的特异性受体,这些位点的单核苷酸多态性为下一步研究探讨FSHR基因对文昌鸡繁殖性能的遗传效应奠定了基础。

文昌鸡FSHR基因多态性及其对繁殖性状的遗传效应

【目的】寻找与文昌鸡繁殖性能相关的遗传标记。【方法】以促卵泡素受体(FSHR)基因作为影响鸡繁殖性状的候选基因,采用PCR-SSCP技术结合测序分析,对FSHR基因所有外显子及部分内含子区域进行单核苷酸多态性(SNPs)检测,收集文昌鸡繁殖性能指标,分析FSHR基因多态性与繁殖性状的关系。【结果】共发现4个区域存在SNPs位点,分别为:区域4中exon 4编码区43bp处的T→C突变,但没有导致翻译后氨基酸序列的改变;区域2中exon 2编码区5′端-49bp处的C→T突变;区域6中exon 6编码区3′端+12bp处的A→G突变;区域9中exon 8编码区3′端+38bp处的G→T突变。对以上4个区域不同基因型与繁殖性状的相关性分析表明,文昌鸡FSHR基因第4外显子呈现的3种基因型(CC/CD/DD)多态性,与文昌鸡300日龄产蛋数及平均联产天数显著相关(P<0.05)),而且CD杂合基因型的300日龄产蛋数及平均联产天数显著高于其他基因型(P<0.05)。【结论】FSHR基因可作为影响文昌鸡产蛋数的候选基因。

莱芜黑山羊卵巢FSHr、LHr的免疫组化定位研究

为从形态学角度理解内分泌调节过程,揭示促性腺激素(GTH)对雌性哺乳动物卵巢调节作用机制,对处于非繁殖季节的莱芜黑山羊卵巢中FSHr、LHr分布进行免疫组化SABC方法定位.分别选取相邻的6张连续阳性切片,光镜观察、图像分析.结果显示:FSHr、LHr阳性细胞主要分布于卵泡颗粒细胞、膜细胞、卵母细胞、血管周围间质,尤其以在卵泡颗粒细胞、膜细胞的胞质中分布最多.原始卵泡卵母细胞中便有两种受体阳性物质分布,在各级卵泡中两种受体阳性细胞数量、染色强度随卵泡发育水平呈正向增加趋势.

子宫内膜息肉组织中FSHR和LHR的表达及意义

目的探讨卵泡刺激素受体(Follicule stimulating hormone receptor,FSHR)、黄体生成素受体(Luteinizing hormone receptor,LHR)与子宫内膜息肉发生的相关性.方法运用实时荧光定量PCR方法(Real-time Quantitative polymerase chain reaction,real-time PCR)以及免疫印迹方法(Southwestern blotting,WB)从基因水平以及蛋白水平测定2016年12月~2017年11月在我院行宫腔镜下子宫内膜息肉摘除术患者子宫内膜息肉及其旁正常子宫内膜中FSHR、LHR的表达差异.结果通过real-time PCR结果显示子宫内膜息肉组织中FSHR基因表达量0.0496(0.0431,0.0656),其旁正常子宫内膜组织中FSHR基因表达量0.0002(0.0001,0.0002),差异有统计学意义(P<0.05);子宫内膜息肉组织中LHR基因表达量(0.00012293±0.00004748),其旁正常子宫内膜组织中LHR基因表达量(0.00001931±0.00000380),差异有统计学意义(P<0.05);通过WB结果显示子宫内膜息肉组织中FSHR蛋白表达水平0.4093(0.3925,0.4789),其旁正常子宫内膜组织蛋白表达水平0.2235(0.1093,0.3285),差异有统计学意义(P<0.05);子宫内膜息肉组织中LHR蛋白表达水平0.4379(0.4062,0.4503),其旁正常子宫内膜组织蛋白表达水平0.2235(0.1093,0.3278),差异有统计学意义(P<0.05).结论 FSHR及LHR存在于人子宫内膜组织中,其在子宫内膜息肉组织中的表达高于其旁正常子宫内膜组织,得出子宫内膜息肉的发生不仅与雌激素受体及孕激素受体表达失调有关,与FSHR及LHR表达失衡亦有关.

LHCGR、FSHR、YAP1DNA多态性与多囊卵巢综合征发病间的相关性研究

目的研究黄体生成素/人绒毛膜促性腺激素受体(LHCGR)、卵泡刺激素受体(FSHR)、Yes相关蛋白1(YAP1)DNA多态性与多囊卵巢综合征(PCOS)发病的相关性。方法选取2019年10月-2021年2月新疆医科大学第一附属医院生殖医学中心PCOS患者59例为PCOS组,以同期健康体检者59例为对照组。采取聚合酶链反应及焦磷酸测序法测定两组LHCGR、FSHR、YAP1DNA多态性,对比两组一般资料及上述基因多态性位点基因型分布频率,采用Logistic回归方程分析PCOS发病的相关因素。结果与对照组比较,PCOS组LH、T指标升高,FSH指标降低,差异有统计学意义(P<0.05);PCOS组rs13405728位点基因型TT、TC、CC频率分别为69.49%、28.81%、1.69%;rs1394205位点基因型AA、AG、GG频率分别为59.32%、22.03%、18.64%;rs11225161基因型AA、AG、GG频率分别为18.64%、59.32%、22.03%;对照组rs13405728位点基因型TT、TC、CC频率分别为50.85%、27.12%、22.03%;rs1394205位点基因型AA、AG、GG频率分别为55.93%、20.34%、23.73%;rs11225161基因型AA、AG、GG频率分别为44.07%、47.46%、8.47%。两组rs13405728位点基因型频率、rs11225161基因型分布频率比较,差异有统计学意义(P<0.05)。结果显示,rs13405728位点基因型、rs11225161位点基因型多态性均与PCOS发生有关(P<0.05)。结论LHCGR、YAP1DNA是PCOS的易感基因,其中rs13405728位点T/C多态、rs11225161位点A/G多态与PCOS易感性存在关联性。

LPS对兔下丘脑、输卵管上FSHR和LHR表达的影响

【目的】检测促卵泡素受体(FSHR)和促黄体素受体(LHR)蛋白在下丘脑、输卵管的分布,以及LPS诱导后母兔下丘脑、输卵管上FSHR和LHR的表达变化。【方法】36只雌性新西兰白兔随机分为9组(n=4),一组不注射作为0h组,LPS处理组按0.5mg/kg体重耳缘静脉注射LPS,对照组注射等量的生理盐水,在注射后0、1.5、3、6和12h后处死,收集下丘脑和输卵管,采用荧光定量PCR和免疫组化在转录水平和蛋白水平分析FSHR和LHR的表达。【结果】结果显示:FSHR和LHR主要定位于输卵管黏膜层和肌层,在间质层未检测到FSHR和LHR;LPS诱导下,LPS不影响FSHR和LHR mRNA在下丘脑的转录,但下调FSHR和LHR mRNA在输卵管的表达。蛋白水平上,LPS改变了FSHR在下丘脑和LHR在输卵管黏膜层的表达模式,对LHR在下丘脑和输卵管肌层有下调作用,对FSHR在输卵管黏膜层和肌层有上调作用。【结论】LPS影响FSHR和LHR蛋白在下丘脑的表达,表明免疫-繁殖系统可以在下丘脑发生相互作用,进而影响动物生殖。

德国牧羊犬FSHR基因第1外显子SNP T89C与产仔数关系研究

为了研究FSHR基因与产仔数的关系,试验以警用德国牧羊犬种母犬基因组为模板,应用PCR技术克隆FSHR基因第1外显子,测序检测单核苷酸多态性(SNP)T89C位点,并进一步分析基因型对产仔数的影响。结果表明:FSHR基因第1外显子SNP T89C CC基因型个体产仔数显著少于TT基因型个体产仔数(P<0.05),说明SNP T89C位点与德国牧羊犬产仔数存在相关性。

北极狐FSHR基因多态性与产仔数关联分析

为了研究北极狐FSHR基因的多态性与北极狐产仔数的相关性,试验采用PCR-SSCP技术检测北极狐FSHR基因多态性,用最小二乘法分析其多态性对北极狐产仔数影响的遗传效应。结果表明:FSHR基因在北极狐中存在多态性,A等位基因为优势等位基因。对于初产母狐,BB基因型母狐的总产仔数(TNB)和产活仔数(NBA)比AA基因型母狐分别多1.08头和1.58头(P<0.05);对于经产母狐,BB基因型母狐的TNB和NBA比AA基因型母狐分别多1.72头和1.03头(P<0.05)。在北极狐群中,北极狐FSHR基因处于Hardy-Weinberg平衡状态。说明北极狐FSHR基因B等位基因对北极狐产仔数性状有显著影响。

阿拉瑞林免疫影响FSHR表达及FSHR生物信息学分析

目的：探讨阿拉瑞林主动免疫绵羊对垂体和卵巢FSHR表达的作用，分析绵羊FSHR的生物信息学特点。方法：42只5～6月龄母绵羊随机分为6组（n＝7），EG-Ⅰ、EG-Ⅱ和EG-Ⅲ分别于0 d和14 d皮下注射阿拉瑞林抗原200μg、300μg和400μg；EG-Ⅳ和EG-Ⅴ分别皮下注射阿拉瑞林抗原200μg、300μg，0、7、14、21 d各一次，共4次；对照组在0 d和14 d皮下注射抗原溶媒2.0ml。于70 d（实验结束时）屠宰动物，无菌采集垂体和卵巢。从绵羊垂体中提取FSH，进行PCR扩增、克隆和测序，荧光定量PCR分析，将得到的序列运用生物信息学软件行分析，用Western blot检测卵巢FSHR蛋白表达。结果：实验组垂体FSHR mRNA的2^-ΔΔCt均低于对照组， EG-Ⅰ、EG-Ⅱ和EG-Ⅲ的2^-ΔΔCt值逐渐下降；而且EG-Ⅳ低于EG-Ⅰ，EG-Ⅴ低于EG-Ⅱ，即注射阿拉瑞林4次后FSHR mRNA的2^-ΔΔCt值分别低于注射2次后的值。各实验组卵巢FSHR蛋白表达量随阿拉瑞林注射剂量的增加而逐渐增加，EG-IV和EG-V卵巢FSHR蛋白显著高于对照组相比（P＜0.01）。 FSHR序列为1091 bp，开放阅读框（0RF）780 bp，位于41～820位点，其半衰期、理论等电点、不稳定指数、疏水性平均值和脂肪指数分别为1.2 h、5.05、47.75、0.836和30.61。结论：阿拉瑞林免疫可抑制垂体FSHR mRNA的表达，但是增加卵巢FSHR蛋白表达；FSHR蛋白为不稳定的疏水性蛋白。

经皮穴位电刺激对IVF中POI患者卵母细胞质量及FSHR表达的影响

目的观察经皮穴位电刺激(TEAS)对体外受精-胚胎移植(IVF-ET)中早发性卵巢功能不全(POI)患者卵母细胞质量及卵泡刺激素受体(FSHR)表达的影响。方法选取2018年5～10月在南方医科大学附属深圳妇幼保健院生殖医学中心接受IVF治疗的POI妇女66例,采用随机数表法分为TEAS组和对照组,每组33例。TEAS组自促性腺激素(Gn)启动日至绒促性素(hCG)注射日给予电子针疗仪治疗,隔日1次,对照组自Gn启动日起给予安慰针治疗,治疗时间、疗程及穴位选择均与TEAS组相同。比较两组患者的获卵数、受精率、优质胚胎率及临床妊娠率的差异,采用Western blot法检测取卵日颗粒细胞FSHR蛋白的表达。结果 TEAS组患者的临床妊娠率为51.52%,明显高于对照组的27.28%,差异有统计学意义(P<0.05);治疗后,TEAS组和对照组的获卵数分别为(3.33±1.05)个、(2.73±1.21)个,优质胚胎率分别为54.29%和34.15%,颗粒细胞FSHR蛋白表达分别为0.75±0.17、0.55±0.12,两组上述指标比较差异均有统计学意义(P<0.05);TEAS组和对照组的受精率分别为75.79%和73.23%,两组比较差异无统计学意义(P>0.05)。结论 TEAS疗法可能通过调控卵巢颗粒细胞FSHR的表达,促进卵母细胞发育,提高卵母细胞质量,改善IVF中POI患者的妊娠结局。

Targeted expression of human FSH receptor Asp567Gly mutant mRNA in testis of transgenic mice: role of humanFSH receptor promoter

Aim: To specifically express the Asp567Gly human follicle-stimulating hormone receptor (FSHR) under the control of its promoter to evaluate the phenotypic consequences in the presence of normal pituitary function. Methods: We produced transgenic mice overexpressing the Asp567Gly human FSHR under the control of a 1.5kb 5' flanking region fragment of its promoter. Results: Mice were phenotypically normal and fertile. In males, mRNA could be detected in the testis and the brain, indicating that the 1.5kb promoter fragment drives expression not only in the gonads. The testis weight/body weight ratio and the testosterone levels in transgenic and non-transgenic litter mates were similar. By in situ hybridisation we found that the transgenic FSHR was highly expressed in Sertoli cells, spermatocytes and round spermatids. However, a radioligand receptor assay failed to show a significant difference in total FSHR binding sites in testis homogenates of transgenic and wild type animals, suggesting that the transgenic FSHR is probably not translated into functional receptor protein. Conclusion: A 1.5kb 5 '-region of the human FSHR drives mRNA expression of the transgene in the testis but leads to ectopic expression in germ cells and in the brain. No phenotypic consequences could be documented due to the lack of protein expression.