Wnt5a抑制Wnt3a促黑素细胞黑素生成的作用探究

目的：研究WntSa对Wnt3a处理过的melan—a细胞分泌黑色素的影响。方法：体外培养黑色素细胞（melan-a细胞）,分别进行GFP、Wnt3a、Wnt3a＋WntSa处理,比较细胞的突起,酪氨酸酶的活性以及黑素合成相关基因（TYR、TRP2、MITF）表达情况。结果：Wnt3a促进黑色素细胞突起的生长和TYR、TRP2、MITF的表达,而Wnt5a逆转了Wnt3a对黑色素细胞的作用。结论：Wnt5a抑制Wnt3a促黑素细胞黑素生成的作用,表明在melan．a黑素细胞中Wnt5a可有效抑制wnt经典通路。     

AFP的亚细胞定位及对肿瘤细胞生长的影响

目的观察甲胎蛋白（AFP）在不同肿瘤细胞中的亚细胞定位及对肿瘤细胞生长的影响。方法运用免疫荧光的方法观察内源性AFP在HeI。a细胞、QGY-7703细胞、MCF-7细胞中的亚细胞定位。将构建的表达AFP的质粒pcDNA3-AFP及AFP腺病毒siRNA干涉载体Adv—AFPsiRNA作用于QGY-7703细胞,MCF-7细胞,运用M1Tr,集落形成实验检测细胞增殖状况。结果免疫荧光显示,内源性的AFP在HeLa细胞、QGY-7703细胞、MCF-7细胞均只在细胞质中表达。pcDNA3-AFP使QGY-7703的细胞活性增加了2l％（P〈0．05）及集落形成能力增加了32％（P〈0．01）,MCF-7实验组比对照组细胞活性降低了30％（P〈0．01）．克隆形成能力降低82％（P〈0．01）。Adv—AFPsiRNA使QGY-7703的细胞活性降低了22％（P〈0．05）,平均克隆形成能力降低52％（P〈0．01）,MCF-7细胞活性提高了24．5％（P〈0．05）,克隆形成能力提高了89％（P〈O．01）。结论内源性的AFP只在细胞质中表达。AFP能促进QGY-7703细胞的增殖及克隆形成能力,而在MCF-7细胞中发挥相反的作用。腺病毒介导的内源性的AFP表达的下调能降低QGY-7703的增殖,却增加了MCF-7的细胞活性及克隆形成能力。     

不同剂量L-酪氨酸（L—TYR）对羊驼黑素细胞增殖及酪氨酸酶mRNA表达的影响

目的：探索不同剂量的L-酪氨酸对羊驼黑素细胞增殖以及酪氨酸酶mRNA表达的影响。方法：体外培养正常羊驼皮肤黑素细胞,显微镜下观察不同剂量的L-酪氨酸（100μmol／L、200μmol／L、300μmol／L、400μmol／L）对羊驼皮肤黑素细胞增殖的影响,利用实时荧光定量PCR技术分析不同剂量L-酪氨酸对酪氨酸酶mRNA的表达量的影响。结果：研究结果显示：在培养的黑素细胞中添加了不同剂量L-酪氨酸3d后,镜检观察,黑素细胞数量相比较空白对照组有所减少,酪氨酸酶mRNA表达量增加且显著高于对照组（P〈0．05）,在200μmol／L时,酪氨酸酶mRNA表达量达到最高峰值。结论：L-酪氨酸能诱导羊驼皮肤黑素细胞酪氨酸酶mRNA表达量增高。     

Wnt5a在增生性瘢痕中的表达及其临床意义

目的：探讨wnt5a在增生性瘢痕中的表达及其临床意义。方法：选择12例增生性瘢痕患者,术中取成熟期增生性瘢痕6份,增殖期增生性瘢痕6份,正常皮肤组织6份。光镜下观察其形态学的差异,通过免疫组化技术检测和比较其Wnt5a阳性表达的细胞面积率。结果：与正常皮肤相比,增殖期增生性瘢痕中有大量的成纤维细胞,胶原纤维含量丰富,且排列紊乱,其间有大量的炎性细胞,成熟期增生性瘢痕也含有丰富的成纤维细胞和胶原,但炎性细胞很少。增殖期增生性瘢痕和成熟期增生性瘢痕组织中真皮浅层和真皮深层Wnt5a阳性表达的细胞面积率均显著高于正常皮肤组织（P〈0．05）,且增殖期增生性瘢痕组织中wnt5a阳性表达的细胞面积率显著高于成熟期增生性瘢痕（P〈0．05）。但正常皮肤组织、成熟期增生性瘢痕、增殖期增生性瘢痕各组间真皮浅层与真皮深层Wnt5a阳性表达的细胞面积率比较均无显著性差异（P〉0．05）。结论：Wnt5a的表达上调可能在增生性瘢痕的形成中起重要作用,并可能与增生性瘢痕的增殖活性有关。     

构建MicroRNA．29a和microRNA-29c腺病毒并探讨其对膀胱癌细胞增殖能力的影响

构建miRNA．29a／c的重组腺病毒并观察其对膀胱癌T24细胞增殖能力的调控。以人全基因组DNA为模板,PcR扩增miR-29a、miR-29c,克隆至腺病毒穿梭载体pAdtrace．TO4-CMV。重组穿梭载体经pmeI线性化后与腺病毒骨架质粒pAdEasy-1共转化感受态大肠杆菌BJ5183,通过同源重组获得重组腺病毒质粒pAdEasy—1—miR-29a、pAdEasy—1．miR-29c,pacI线性化后转染HEK-293细胞,进行包装和扩增。实时荧光定量PcR检测感染腺病毒的膀胱癌T24细胞miR-29a、miR．29c的表达水平,并利用CCK．8实验检测细胞增殖能力。经DNA测序和限制性内切酶分析显示,重组腺病毒质粒pAdEasy—1—miR．29a、pAdEasy．1-miR-29c构建成功：感染腺病毒Ad—miR-29a和Ad—miR．29c后,经实时荧光定量PCR检测,膀胱癌细胞中miR．29a、miR．29c表达显著增高（P〈0．01）;过表达miR．29a／c后的CCK．8实验显示,细胞增殖能力明显低于对照组伊〈0．05）。以上说明已成功构建miR．29a、miR．29c腺病毒,过表达miR．29a／c可抑制膀胱癌细胞的增殖。     

他卡西醇对人黑素细胞生物学性状的影响

目的:观察他卡西醇对体外培养的正常人黑素细胞增殖、黑素合成及酪氨酸酶(TYR)mRNA表达、酪氨酸酶相关蛋白-1(TRP-1)mRNA表达的影响,探讨他卡西醇治疗白癜风的机制.方法:体外黑素细胞培养,给予不同浓度他卡西醇(10-6、10-7、10-8、10-9、10-10mol/L)处理,用MTT法测定细胞增殖,碱裂解法测定黑素合成,多巴氧化法检测酪氨酸酶活性,半定量RT-PCR法检测TYR、TRP-1 mRNA的表达.结果:10-8 mol/L他卡西醇能刺激黑素细胞增殖,10-8、10-9 mol/L能促进黑素合成,10-9～10-6 mol/L的他卡西醇能显著增强正常人黑素细胞酪氨酸酶活性并上调TYR、TRP-1mRNA的表达.结论:他卡西醇可促进黑素细胞增殖,并提示该药物可能通过上调酪氨酸酶家族中关键基因TYR、TRP-1mRNA的表达来提高酪氨酸酶活性,最终增加黑素合成.     

KI对l染铅近曲肾小管上皮细胞I A 表达及凋亡的影响

目的：研究碘化钾对染铅肾小管上皮细胞XIAP的表达及凋亡的影响,探讨其对抵抗铅导致的近曲肾小管上皮细胞损伤的可能机制。方法：应用流式细胞术检测染铅HK-2细胞及对照组细胞中XIAP的表达及凋亡情况。结果：染铅HK-2细胞中XIAP的表达明显低于对照组,且虽然铅浓度的增高而降低（P〈0．05／P〈0．01）,碘化钾能够减弱上述变化（P〈0．05／P〈0．01）;染铅HK-2细胞的凋亡率明显高于对照组,且虽然铅浓度的增高而升高（P〈0．05／P〈0．01）,碘化钾能够降低染铅细胞的凋亡率（P〈0．05／P〈0．01）。结论：碘化钾能够上调染铅HK-2细胞中抗凋亡蛋白XIAP的表达,降低凋亡率,在一定程度上降低铅对细胞的损伤。     

高糖诱导腹膜间皮细胞发生上皮问质转化中microRNA的异常变化

目的：定腹膜间皮细胞在高糖引起上皮间质转化（Epithelial—mesenchymnal transition,EMT）过程中microRNA的表达差异。方法：常规培养PMC细胞,利用高糖培养液刺激诱导腹膜间皮细胞发生EMT,倒置显微镜观察各组细胞形态学变化,实时定量PCR检测EMT标志基因变化,以此确定高糖诱导EMT的发生。利用特异茎环结构的引物合成microRNA的cDNA,实时定量PCR检测重要microRNA的表达变化。结果：高糖培养液培养腹膜间皮细胞48hr后,细胞形态呈梭形改变,同时EMT标记基因E—cadherin表达明显减低（P〈0．01）,Vimentin表达显著升高（P〈0．01）,说明高糖诱导腹膜间皮细胞发生了EMT。利用microRNA特异的茎环结构引物,实时定量PCR检测结果发现高糖刺激后miR-193a的表达明显上调（P〈0．01）;miR-15a和let-7e的表达明显降低（P〈0．01）;miR-16和miR-21的表达无明显变化（P〉0．05）,同时检测发现高糖刺激后miR-193a的表达水平随刺激时间表达升高。结论：异常变化的microRNA可能对高糖诱导的腹膜间皮细胞EMT具有重要调控作用。     

SFRP4抑表达对HT-29细胞侵袭能力的影响

目的：观察SFRP4对HT29细胞侵袭转移能力的影响。方法：以HT29细胞为研究对象,SFRP4siRNA通过脂质体转染HT29细胞,westernblot检测HT29细胞中wnt、细胞核β—Catenin蛋白的表达、elisa法检测细胞培养上清MMP-2、MMP．9的含量,Transwell小室观察成的转移侵袭能力。结果：干扰SFRP4后能显著降低HT29细胞中Wnt、细胞核中B—Catenin蛋白的表达、细胞培养上清MMP-2、MMP-9的含量,（P〈0．01）,降低HT29细胞的转移侵袭能力（P〈0．01）。结论：抑制SFRP4表达能抑制HT29细胞的转移侵袭,其机制可能与抑制HT29细胞wnt信号通路有关。     

West Nile Virus (WNV) protease and membrane interactions revealed by NMR spectroscopy

Although the importance of Wnt3a in melanocyte development has been well recognized, the effect of Wnt3a in normal HF melanocytes has not been clearly elucidated yet. Thus, we sought to examine the presence and location of Wnt3a in HF during hair cycle. By using melanocyte-targeted Dct-LacZ transgenic mice, we found that Wnt3a signaling is activated in mouse HF melanocytes during anagen of hair cycle. To further explore the potential functions of Wnt3a in mouse melanocytes, we infected melan-a cells with AdWnt3a to serve as the production source of Wnt3a protein. We demonstrated that Wnt3a promoted melanogenesis through upregulation of MITF and its downstream genes, tyrosinase and TRP1, in melanocytes. In vivo, AdWnt3a rescued the effects of AdsimMITF on HF melanocytes and promoted melanin synthesis. Our results suggest that Wnt3a plays an important role in mouse HF melanocytes homeostasis.     

G1对EA.hy926内皮细胞内质网应激的抑制作用

目的观察GPR30受体激动剂G1对高糖诱导的EA.hy926内皮细胞内质网应激(endoplasmic reticulum stress,ERS)的影响。方法选用EA.hy926内皮细胞为研究对象,分为3组:正常对照组(Con,17.51mmol/L葡萄糖)、高糖组(HG,33.3mmol/L葡萄糖)、高糖+G1组(HG+G1,HG+1umol/L G1),利用流式细胞术检测3组细胞凋亡率,Western blot法检测ERS相关分子Bip、IRE1、PERK及凋亡分子Bax、Bcl-2的表达变化,RT-PCR法检测Bip和CHOP的mRNA表达变化。结果 HG组与Con组比较,细胞凋亡率明显升高(P0.01),Bip、IRE1、PERK及凋亡分子Bax表达上调(P0.01,P0.05或P0.001),Bcl-2的表达下调(P0.01),Bip mRNA、CHOP mRNA表达上调(P0.001及P0.01);HG+G1组与HG组比较,细胞凋亡率明显降低(P0.05),Bip、IRE1、PERK及凋亡分子Bax表达下调(P0.05或P0.01),Bcl-2的表达上调(P0.05),Bip mRNA、CHOP mRNA表达下调(P0.001及P0.01)。结论 GPR30受体激动剂G1可抑制EA.hy926内皮细胞内质网应激。     

长期酒精摄入对雄性大鼠生殖系统的损伤

目的：研究长期酒精摄入对雄性大鼠生殖系统的损伤机制。方法：选用8周龄的SD大鼠,进行随机分组：对照组（5％蔗糖,口服）;酒精组（4g／kg,口服）。连续12周后,分别取附睾考察精子数目、活力;取血清检测睾酮和促黄体生产素（LH）含量;计算睾丸一体重比,并检测睾丸中丙二醛（MDA）、谷胱甘肽（GSH）含量以及谷胱甘肽过氧化物酶（GPx）和超氧化物歧化酶（SOD）的活性;同时检测凋亡相关蛋白bax,bcl-2以及caspase．3前体和剪切体的蛋白表达。结果：酒精组12周后,大鼠的睾丸．体重比明显降低（P〈0．05）,精子数目减少（P〈0．01）,精子活力下降（P〈0．01）;血清中睾酮含量下降（P〈0．05）,LH含量增加（P〈0．05）;睾丸中MDA含量增加（P〈0．01）,GSH含量降低（P〈0．05）,GPX和SOD活性下降（P〈0,01）;凋亡相关蛋白bax表达增加（P〈0．05）,caspase-3剪切体与前体的比值增加（P〈O．01）。结论：长期摄入酒精引起的大鼠睾丸内氧化应激水平的增加是其导致其生殖系统损伤的重要因素之一。     

DKK3调控羊驼黑色素细胞中黑色素生成

Dickkopf-3(DKK3),Wnt/p-catenin信号通路中一个重要的抑制因子,可能参与调控黑色素生成过程.本文研究了DKK3在羊驼黑色素细胞中黑色素生成的作用.在羊驼黑色素细胞中,过表达DKK3显著下调Wntl,Lefl,Myc和黑色素生成相关基因MITF及其下游基因TYR,TYRP1和TYRP2的表达,在...     

Wnt inhibitory factor (WIF)‐1 promotes melanogenesis in normal human melanocytes

Wnt signaling plays a role in the differentiation as well as the development of melanocytes. Using a microarray analysis, hyperpigmentary skin of melasma expressed high levels of Wnt inhibitory factor‐1 (WIF‐1) compared with perilesional normal skin. In this study, the expression and functional roles of WIF‐1 on melanocytes were investigated. WIF‐1 was expressed both in the melanocytes of normal human skin and in cultured melanocytes. The upregulation of WIF‐1 on cultured normal human melanocytes significantly induced expressions of MITF and tyrosinase, which were associated with increased melanin content and tyrosinase activity. Consistent with the stimulatory effect of WIF‐1, WIF‐1 siRNA reduced melanogenesis in the cells. Moreover, WIF‐1 increases pigmentation in melanocytes co‐cultured with WIF‐1‐overexpressed fibroblasts and of organ‐cultured human skin. These findings suggest that melanocytes express WIF‐1 constitutively in vivo and in vitro and that WIF‐1 promotes melanogenesis in normal human melanocytes.     

The etiology of oculocutaneous albinism (OCA) type II: the pink protein modulates the processing and transport of tyrosinase

Oculocutaneous albinism (OCA) is caused by reduced or deficient melanin pigmentation in the skin, hair, and eyes. OCA has different phenotypes resulting from mutations in distinct pigmentation genes involved in melanogenesis. OCA type 2 (OCA2), the most common form of OCA, is an autosomal recessive disorder caused by mutations in the P gene, the function(s) of which is controversial. In order to elucidate the mechanism(s) involved in OCA2, our group used several antibodies specific for various melanosomal proteins (tyrosinase, Tyrp1, Dct, Pmel17 and HMB45), including a specific set of polyclonal antibodies against the p protein. We used confocal immunohistochemistry to compare the processing and distribution of those melanosomal proteins in wild type (melan-a) and in p mutant (melan-p1) melanocytes. Our results indicate that the melanin content of melan-p1 melanocytes was less than 50% that of wild type melan-a melanocytes. In contrast, the tyrosinase activities were similar in extracts of wild type and p mutant melanocytes. Confocal microscopy studies and pulse-chase analyses showed altered processing and sorting of tyrosinase, which is released from melan-p1 cells to the medium. Processing and sorting of Tyrp1 was also altered to some extent. However, Dct and Pmel17 expression and subcellular localization were similar in melan-a and in melan-p1 melanocytes. In melan-a cells, the p protein showed mainly a perinuclear pattern with some staining in the cytoplasm where some co-localization with HMB45 antibody was observed. These findings suggest that the p protein plays a major role in modulating the intracellular transport of tyrosinase and a minor role for Tyrp1, but is not critically involved in the transport of Dct and Pmel17. This study provides a basis to understand the relationship of the p protein with tyrosinase function and melanin synthesis, and also provides a rational approach to unveil the consequences of P gene mutations in the pathogenesis of OCA2.     

过表达ER恢复雌激素对子宫内膜癌KLE细胞中Notch信号通路的调控

目的：通过观察雌激素对子宫内膜癌KLE细胞中Notch信号通路的影响,探讨过表达雌激素核受体（estrogenreceptor,ER）是否可以恢复雌激素对Notch信号通路的调控作用,继而调节细胞增殖活性。方法：MTT检测雌激素及Notch信号通路对细胞增殖活性的影响;RT．PCR及Westem．blotting检测雌激素及Notch通路抑制剂DAPT对Notch表达的影响;质粒的抽提及转染使KLE细胞中的雌激素核受体ER过表达。结果：雌激素呈剂量依赖效应促进KLE细胞的增殖活性,其中以雌激素浓度为1．0×10-9M时最明显（相对于对照组为1．25±0．026,P〈0．05）;抑制Notch信号通路的表达可以明显下调KLE细胞的增殖活性（0．76±0．02,P〈0．05）;在KLE细胞中,雌激素对Notch的表达没有明显的调控作用,但是将其雌激素核受体过表达后,雌激素可明显上调Notch的表达,并显著促进细胞的增殖活性（1．24±0．02,P〈0．05）。结论：在ER阴性的子宫内膜癌细胞中过表达ER,可以恢复雌激素对Notch信号通路的调控,从而进一步的调控细胞增殖活性。     

EGCG对LPS刺激人肺腺癌A549细胞凋亡及CUGBP1蛋白表达的影响

目的：研究表没食子儿茶素-3-没食子酸酯（epigallocatechin-3-gallate,EGCG）对炎性刺激的人肺腺癌A549细胞增殖和凋亡的影响及与CUGBP1表达的关系。方法：MTT法检测EGCG和LPS刺激A549细胞增殖活性的影响;流式细胞仪检测细胞凋亡;免疫细胞化学检测EGCG对LPS刺激人肺腺癌A549细胞内CUGBP1蛋白的表达。结果：与对照组相比,LPS体外显著促进A549细胞增殖,其胞核胞质内CUGBP1表达明显增强（P〈0.01）。加入EGCG可拮抗LPS促A549细胞增殖的作用,促进其凋亡,明显抑制LPS刺激的A549细胞内CUGBP1的表达（P〈0.01）。CUGBP1蛋白定量分析可知EGCG和LPS共同孵育A549细胞4h、24h时,细胞中的CUGBP1蛋白表达量较单纯LPS作用时降低。但EGCG和LPS共同孵育A549细胞24h,A549细胞中胞核CUGBP1蛋白表达量（1210.565±3.46）较4h时胞核CUGBP1蛋白表达量（67.344±3.68）高,差异有统计学意义（t=927.164,P〈0.001）。结论：EGCG可能通过干扰CUGBP1基因的表达抑制炎症刺激人肺腺癌细胞A549的增殖,促进其凋亡。