CDK_4I/MTS_1基因产物P_16^(INK4A)及其与P_(Rb)及P_(53)的关系

随着细胞遗传学及分子生物学技术的日臻完善,人们发现在细胞发生恶性转化的过程中,除癌基因/抑癌基因的正负调节失控外,许多细胞周期中的内外因子参与了这一过程.目前,较引人注目的就是1994年美国报道的位于人类染色体9P_(21)的P_(16)^(INK4A)基因,又称CDK_4I(Cylin-dependent Kinase4 inhibitor)或MTS_1(multipletumor suppressor genel),编码15.84KI的蛋白产物.作为CDK4的抑制因子,抑制细胞的分裂.P_(16)^(INK4A)基因的纯合子丢失在5O%～85%的人类肿瘤,如肺癌、乳腺癌、膀胱癌、肾癌、皮肤癌及白血病的细胞系中得到了证实.众多的研究提示P_(16)基因可能是9P_(21)区域的候补肿瘤抑制基因.人们也注意到它的表达水平在一些类型的肿瘤中与公认的作用于G_1期的抑癌基因产物P_(Rb)

人黑色素瘤细胞系MTS1/p16CDDK4基因的突变

为了探讨p16基因在人肿瘤细胞系中的突变,采用PCR-SSCP分析和基因序列测定技术,对人黑色素瘤细胞系(Bowes)中p16基因的突变进行检测。结果显示,Bowes细胞的p16基因第二外显子扩增产物在聚丙烯酰胺凝胶中电泳异常,表明其基因序列存在点突变。核酸序列测定证实第341号核苷酸发生T→C的颠换。应用DNA重组技术构建的突变型p16基因重组质粒可作为基因探针用于检测p16基因的缺失。

胃癌中p16基因表达、缺失及突变的检测

目的:研究p16基因表达与胃癌发生发展、侵袭、转移的关系及p16基因外显子2缺失、突变在胃癌发生中的地位。方法:运用链霉菌抗生物素蛋白-过氧化酶SP免疫组织化学方法检测胃癌及癌前病变组织中p16蛋白的表达;采用聚合酶链反应PCR、聚合酶链反应-单链构象多态性PCRSSCP分析方法检测胃癌中p16基因外显子2的缺失、突变。结果:1p16蛋白表达阳性率:①正常胃粘膜96.25%77/80,不典型增生92.00%45/50,胃癌47.54%58/122,胃癌组中p16蛋白表达低于正常胃粘膜及不典型增生(P<0.05);②粘液腺癌10.00%,1/10低于低分化腺癌51.22%,21/41、未分化癌57.69%,15/26和印戒细胞癌62.50%,10/16(P<0.05);③30例原发癌和淋巴结转移癌配对标本中p16蛋白表达阳性率:原发癌46.67%(14/30),淋巴结转移癌16.67%5/30,淋巴结转移癌低于原发癌P<0.05;2p16基因缺失与突变分析:25例胃癌中检测出缺失5例但未发现突变。结论:①p16蛋白表达缺失与胃癌的发生、组织学类型及淋巴结转移有关。②p16基因外显子2缺失可能与胃癌发生有关而p16基因突变可能与胃癌发生无关。

Hela细胞P16^(ink4)cDNA的克隆及序列分析

P16^(ink4)是CDK抑制蛋白,参与调控细胞G1期至S期的转换。目前发现P16`(ink4)基因损伤与多种肿瘤的发生、发展有关,可能是功能上非常重要的抑癌基因。为了研究该基因的功能,以及突变对该基因功能的影响,本文应用RT-PCR方法,从Hela细胞中克隆了P16^(ink4)cDNA。扩增得到556bp片段(包括引物两端酶切位点的16bp)克隆于M13载体,测定了其DNA序列。该序列包括了P16^(ink4)cDNA编码区全部471bp,以及3’端69bp序列。表明P16^(ink4)cDNA已成功地得到克隆。

P16基因甲基化与消化系统恶性肿瘤

P16基因又称多肿瘤抑制因子1(MTS1)、CDK4抑制因子(NK4)，是1993年发现并克隆出的一个参与细胞周期调控的抑癌基因。由于其作用和重要性不亚于P53基因，因而成为近年来研究的热点。

Expression,deleton and mnutation of ρ16 gene in human gastric cancer

AIM To investigate the relationship between the expression of p16 gene and the gastric carcinogenesis,depth of invasion and lymph node metastases, and to evaluate the deletion and mutation of exon 2 in p16 gene in gastric carcinoma.METHODS The expression of P16 protein was examined by streptavidin-peroxidase conjugated method (S-P); the deletion and mutation of p16 gene were respectively examined by polymerase chain reaction (PCR) and polymerase chain reaction single-strand conformation polymorphism analysis (PCR-SSCP) in gastric carcinoma.RESULTS Expression of P16 protein was detected in 96.25% (77/80) of the normal gastric mucosa, in 92.00% (45/50) of the dysplastic gastric mucosa and in 47.54% (58/122) of the gastric carcinoma. The positive rate of P16 protein expression in gastric carcinoma was significantly lower than that in normal gastric mucosa and dysplastic gastric mucosa (P＜0.05). The positive rate of P16 protein expression in mucoid carcinoma 10.00% (1/ 10) was significantly lower than that in poorly differentiated carcinoma 51.22% ( 21/ 41 ),undifferentiated carcinoma 57.69% (15/26) and signet ring cell carcinoma 62.50% (10/ 16) (P＜0.05). The positive rate of p16 protein in 30 cases paired primary and lymph node metastatic gastric carcinoma: There was 46.67% (14/30) in primary gastric carcinoma, 16.67% (5/30) in lymph node metastatic gastric carcinoma. The positive rate of lymph node metastatic carcinoma was significantly lower than that of primary carcinoma (P＜0.05). There was of p16 gene mutation in exon 2, but 5 cases displayed deletion of p16 gene in exon 2 in the 25 primary gastric carcinomas.CONCLUSIONS The expression loss of P16 protein related to the gastric carcinogenesis, gastric carcinoma histopathological subtypes and lymph metastasis. The mutation of p16 gene in exon 2 may not be involved in gastric carcinogenesis. But the deletion of p16 gene in exon 2 may be involved in gastric carcinogenesis.