淫羊藿苷对维生素D缺乏大鼠肾上腺皮质维生素D轴及VDR蛋白表达的影响

目的：观察淫羊藿苷对维生素D缺乏大鼠肾上腺皮质维生素D轴的影响。方法：选用60只雄性SD大鼠,随机分为：正常组;模型组（生理盐水4.0 mL·kg-1·d-1灌胃）;淫羊藿苷高剂量组（120 mg·kg-1·d-1灌胃）;淫羊藿苷中剂量组（60 mg·kg-1·d-1灌胃）;淫羊藿苷低剂量组（30 mg·kg-1·d-1灌胃）;维生素D组（30ng·kg-1·d-1灌胃）。造模1月后,药物干预2月,酶联免疫法（ELISA法）检测血清25（OH）D3、1,25（OH）D3。免疫组化检测VDR蛋白表达。Real-Time PCR法检测肾上腺皮质维生素D受体（VDR）、25-羟维生素D3-24-羟基化酶（CYP24A1）、25-羟维生素D1α-羟化酶（CYP27B1）mRNA表达。结果：与正常组比较,模型组血清25（OH）D3、1,25（OH）D3含量下降（P〈0.05）;淫羊藿苷干预后血清25（OH）D3、1,25（OH）D3含量均上升（P〈0.05）。免疫组化显示,与正常组比较,模型组VDR蛋白表达下降（P〈0.05）;经淫羊藿苷干预后,表达上升（P〈0.05）。Real-Time PCR显示,经淫羊藿苷干预后,表达量上调（P〈0.05）,除VDRmRNA外,CYP24A1mRNA与CYP27B1mRNA变化趋势均与维生素D组表现一致。模型组基因表达均高于正常组（P〈0.05）,Real-Time PCR检测结果与免疫组化检测的蛋白表达不完全一致。结论：淫羊藿苷可能调节维生素D轴促进VDR蛋白表达改善维生素D缺乏。

Immunohistochemical evaluation of vitamin D receptor(VDR) expression in cutaneous melanoma tissues and four VDR gene polymorphisms

Objective:Vitamin D receptor(VDR)mediates vitamin D activity.We examined whether VDR expression in excised melanoma tissues is associated with VDR gene(VDR)polymorphisms.Methods:We evaluated VDR protein expression(by monoclonal antibody immunostaining),melanoma characteristics,and carriage of VDR-Fok I-rs2228570(C>T),VDR-Bsm I-rs1544410(G>A),VDR-ApaI-rs7975232(T>G),and VDR-TaqI-rs731236(T>C)polymorphisms(by restriction fragment length polymorphism).Absence or presence of restriction site was denoted by a capital or lower letter,respectively:"F"and"f"for Fok I,"B"and"b"for Bsm I,"A"and"a"for ApaI,and "T"and"t"for TaqI endonuclease.Seventy-four Italian cutaneous primary melanomas(52.1±12.7 years old)were studied;51.4% were stage Ⅰ,21.6% stage Ⅱ ,13.5% stage Ⅲ,and 13.5% stage Ⅳ melanomas.VDR expression was categorized as follows:100% positive vs.<100%;over the median 20%(high VDR expression)vs.≤20%(low VDR expression);absence vs.presence of VDR-expressing cells.Results:Stage I melanomas,Breslow thickness of<1.00 mm,level II Clark invasion,Aa heterozygous genotype,and AaTT combined genotype were more frequent in melanomas with high vs.low VDR expression.Combined genotypes BbAA,bbAa,AATt,BbAATt,and bbAaTT were more frequent in 100%vs.<100%VDR-expressing cells.Combined genotype AATT was more frequent in melanomas lacking VDR expression(odds ratio=14.5;P=0.025).VDR expression was not associated with metastasis,ulceration,mitosis>1,regression,tumor-infiltrating lymphocytes,tumoral infiltration of vascular tissues,additional skin and non-skin cancers,and melanoma familiarity.Conclusions:We highlighted that VDR polymorphisms can affect VDR expression in excised melanoma cells.Low VDR expression in AATT carriers is a new finding that merits further study.VDR expression possibly poses implications for vitamin D supplementation against melanoma.VDR expression and VDR genotype may become precise medicinal tools for melanoma in the future.

VDR和GLi1在前列腺癌细胞PC-3中的表达及其相关性

目的初步探讨慢病毒携带sh RNA-VDR载体干扰前列腺癌PC-3细胞中VDR基因对GLi1的影响。方法依照PC-3细胞的培养条件培养细胞;采用荧光定量PCR法和免疫细胞化学SP法检测PC-3细胞中VDR、GLi1两个基因表达情况;对PC-3细胞病毒侵染进行效率评价;运用RT-PCR法检测PC-3细胞VDR基因干扰效果及Gli1转录水平改变情况。结果细胞培养:拍照记录细胞状态:PC-3细胞生长状态良好,以4 d为1周期进行传代;荧光定量PCR法和免疫细胞化学SP法显示VDR、GLi1均在PC-3细胞中表达;慢病毒侵染效率显示为按照1∶10的比例向PC-3细胞加入LV3-NC慢病毒时,细胞侵染效率最好,约为95%左右;RT-PCR显示:VDR-sh RNA慢病毒成功干扰VDR表达,在VDR-sh RNA慢病毒转染72 h后与对照组相比实验组VDR基因转录水平下降85%(P<0.05),同时实验组GLi1基因转录水平与对照组相比上升9%(P<0.05);而当转染96 h后实验组VDR基因转录水平与对照组相比下降99%(沉默),同时实验组GLi1基因转录水平与对照组相比上升248%(P<0.05)。结论所培养的PC-3细胞状态较好;VDR和GLi1基因在PC-3细胞中均表达;慢病毒按照1∶10的比例侵染PC-3效率最高;当VDR被干扰后GLi1表达增高,因而在前列腺癌细胞中维生素D可抑制Hh信号通路可致GLi1表达下调。

酵母双杂交筛选与小鼠维生素D受体互作的蛋白

通过酵母双杂交实验技术筛选小鼠VDR相互作用的蛋白质,评价不同蛋白与VDR的结合活性,以期获得基于互作影响雄性生殖能力基因。扩增小鼠VDR完整CDS序列,克隆至诱铒表达载体pGBKT7,经菌落PCR、DNA测序鉴定,获得重组载体pGBKT7-VDR。随后将重组载体转化至酿酒酵母AH109,并进行毒性和自激活检测;然后与含小鼠cDNA文库的Y187酵母杂交,获得阳性克隆,经HindⅢ酶切,测序分析VDR互作候选蛋白的核酸序列,再检测β-半乳糖苷酶活性,评价候选蛋白与VDR作用力的强弱。结果表明,从小鼠cDNA文库中获得12个与VDR互作的候选蛋白。初步检测到12个蛋白可能与VDR互作,其中3个蛋白因子可能与VDR结合并调控蛋白激酶磷酸化或去磷酸化以影响精子形成、发育和精子活力。