人脑星形细胞瘤中p27 kip1 蛋白和增殖细胞核抗原PCNA 表达的变化

目的:研究p27kip1蛋白和增殖细胞核抗原(proliferating cell nuclear antigen,PCNA)在星形细胞瘤中的表达与肿瘤病理分级的关系,探讨p27kip1蛋白在星形细胞瘤演变过程中的意义。方法:SP免疫组化法对64例星形细胞瘤的p27kip1蛋白和PCNA表达进行观察。结果:随着病理级别的升高,p27kip1阳性细胞百分率降低,而PCNA则相反,两者的表达成显著负相关。结论:p27kip1表达的缺失可能与星形细胞瘤的发生发展密切相关,PCNA能较客观地反映肿瘤的恶性程度。     

p27kip1、Cyclin D1在卵巢癌中的表达及临床意义

目的探讨p27kip1、Cyclin D1在卵巢癌发生方面的意义.方法应用免疫组织化学方法及半定量分析方法,检测50例卵巢癌、19例卵巢良性上皮肿瘤、 13例正常卵巢组织中的p27kip1和Cyclin D1表达,并分析它们与良恶性肿瘤、病理学分级、临床分期的相关性. 结果正常卵巢和卵巢良性肿瘤间,p27和Cyclin D1的各自表达无明显差异;p27在正常卵巢组织和卵巢良性上皮肿瘤中高表达,在卵巢癌中表达降低(P<0.05),且随着肿瘤分级、分期增高(恶性程度增高),阳性表达率逐渐下降;而Cyclin D1的表达则相反;两者在肿瘤中的表达呈负相关.结论 p27kip表达下降、Cyclin D1过表达可能在卵巢癌的发生中起重要作用,检测p27kip1、Cyclin D1在卵巢癌中的表达可预测肿瘤生物学行为特征,可以作为判断预后的指标.     

p27kip1蛋白在胶质瘤细胞中的表达及定位研究

目的：探讨胶质瘤细胞中p27酬蛋白的表达、定位,为进一步研究p27kip1在胶质瘤发生、发展过程中的功能奠定理论基础。方法：用免疫荧光方法检测U87、LN308细胞p27kiP1蛋白的定位情况;进一步分离两种细胞的细胞质与细胞核,在显微镜下观察细胞核形态并用DAPI染色分析细胞核完整性,提取蛋白用Westernblotting。方法检测分离的细胞质与细胞核蛋白的纯度,并检测p27kip1,在细胞中的表达情况。结果：成功分离了细胞的细胞浆与细胞核,并得到纯度较好的细胞浆蛋白与细胞核蛋白。确定了p27kip1蛋白主要表达于U87和LN308细胞的细胞质中。结论：p27kip1蛋白在恶性胶质瘤中可能主要表达在细胞质中,并且其亚细胞定位可能与胶质瘤的恶性程度相关。     

p27kip1基因纳米粒子抑制鼠移植静脉内膜增殖的实验研究

用美国FDA批准使用的生物可降解材料聚乳酸聚乙醇酸共聚物 (PLGA) 为载体材料,制备载p27kip1基因的纳米粒子. 用激光光散射法测定纳米粒子的平均粒径为288.9 nm,粒径呈窄分布,扫描电镜观察纳米粒子表面光滑. DNA含量为3%. 包封效率为86%. 观察p27kip1基因纳米粒子的体外释放情况,发现DNA体外最初释放速度较大,约1周后释放速度开始减缓,可维持平稳释放15天以上. 体外转染大鼠血管平滑肌细胞,用流式细胞仪检测到p27kip1基因纳米粒子对细胞周期进程的抑制作用. 建立自体静脉移植大鼠模型,随机分成三组进行试验：p27kip1基因纳米粒子组,空白纳米粒子组,单纯静脉移植组. 分别于给药后3天、7天、14天、28天取材,HE染色及Verhoeff 染色检测内膜厚度,蛋白质印迹检测P27抑癌基因蛋白的表达,免疫组化SABC法检测移植静脉内膜PCNA、E2F表达. 动物模型试验中转基因组内膜平均厚度较其他组明显减少 (P < 0.01);转基因组PCNA的表达较其他组明显降低 (P < 0.01);转基因组E2F的表达7 ~ 14天较其他组显著降低 (P < 0.01);对照组及单纯静脉移植组之间均无明显差异. 纳米粒子作为p27kip1基因载体能够有效抑制自体静脉移植后内膜平滑肌细胞的增殖.     

p27~(kip1)及相关分子skp2在肺癌组织中的表达及其临床意义

目的:研究细胞周期素依赖性激酶抑制蛋白27(p27kip1)和细胞S相激酶相关蛋白2(skp2)在肺癌癌组织中的表达及意义。方法:选取于我院就诊的72例肺癌患者的肺癌组织和20例癌旁正常肺组织,采用免疫组化技术检测标本中p27kip1和skp2的表达,并分析其与患者的临床病理之间的关系。结果:skp2在肺癌组织中的表达高于正常肺组织,而p27kip1在肺癌组织中的表达低于正常肺组织,差异均有统计学意义(P0.05),且两者的表达呈负相关关系,相关系数r=-0.855(P0.05),skp2的表达与肺癌组织学类型、分化程度、TNM分期、淋巴结有无转移、吸烟与否及p27kip1蛋白表达有关(P0.05)。结论:p27kip1低表达和skp2高表达可能是肺癌发生发展的重要原因,可应用于临床诊治肺癌患者和判断预后。     

人脑星形细胞瘤中p53，Fas／FasL的表达及其与凋亡关系的研究

目的：探讨细胞凋亡在星形细胞瘤中的作用及其与p53、Fas和Fas配体（Fas ligand,FasL）的关系。方法：对43例星形细胞瘤的标本分别进行HE染色,TUNEL及免疫组化分别标记p53,Fas和FasL。结果：高级别肿瘤和低级别肿瘤间的凋亡无显著差异（P〉0．05）。高级别星形细胞瘤的p53,Fas和FasL的表达均显著高于低级别肿瘤（P均〈0．05）。结论：突变型p53可作为评价星形细胞瘤生物学行为的参考指标。与低级别星形细胞瘤相比,高级别肿瘤中的细胞凋亡受到了抑制,且Fas与FasL的过表达对细胞凋亡可产生明显影响。     

人脑星形细胞瘤中p53，Fas/FasL 的表达及其与凋亡关系的研究

目的:探讨细胞凋亡在星形细胞瘤中的作用及其与p53、Fas和Fas配体(Fas ligand,FasL)的关系。方法:对43例星形细胞瘤的标本分别进行HE染色,TUNEL及免疫组化分别标记p53,Fas和FasL。结果:高级别肿瘤和低级别肿瘤间的凋亡无显著差异(P>0.05)。高级别星形细胞瘤的p53,Fas和FasL的表达均显著高于低级别肿瘤(P均<0.05)。结论:突变型p53可作为评价星形细胞瘤生物学行为的参考指标。与低级别星形细胞瘤相比,高级别肿瘤中的细胞凋亡受到了抑制,且Fas与FasL的过表达对细胞凋亡可产生明显影响。     

HIV-1 p24和SIV p27两种ELISA试剂盒检测SIV p27抗原的比较

目的由于检测SIV p27抗原试剂盒来源困难,有时不稳定,鉴于HIV-1 p24与SIVp27有较强的交叉抗原,本研究比较HIV-1 p24和SIV p27两种ELISA试剂盒检测SIV p27抗原得出的结果是否存在一定的相关性。方法 HIV-1 p24和SIV p27两种ELISA试剂盒定性和定量检测样品中SIV p27抗原,并对检测结果进行回归和相关分析。结果 HIV-1 p24和SIV p27两种ELISA试剂盒检测SIV p27抗原的灵敏度分别是150 pg/mL和62.5 pg/mL。两种试剂盒检测病毒液和血浆中SIV p27抗原的定性结果一致。定量结果的统计分析得出病毒液的直线回归决定系数R2=0.857,直线相关系数r=0.926,P〈0.01,直线正相关程度较高;血浆的直线回归决定系数R2=0.512,直线相关系数r=0.716,P〈0.05,直线正相关程度较低。结论 HIV-1 p24 ELISA试剂盒能够替代SIVp27 ELISA试剂盒定性检测病毒液和血浆中SIV p27抗原,但只能定量检测病毒液中SIV p27抗原。     

肺癌中增殖细胞核抗原表达、DNA含量测定及其与预后的关系

本文采用ＳＰ免疫组织化学方法对６７例肺癌进行增殖细胞核抗原染色、与图像分析技术测定ＤＮＡ含量作相关性分析,探讨其在判断肺癌预后方面的意义。结果：（１）ＰＣＮＡ阳性表达强度与预后明显相关。（２）肺癌组织中ＰＣＮＡ表达强度与ＤＮＡ含量之间存在较好的相关性。（３）肺癌组织中多倍体随ＰＣＮＡ表达增强而增多,二倍体则随ＰＣＮＡ表达增强而减少。说明用简单的免疫组织化学方法检测肺癌组织中ＰＣＮＡ,以此来观察肿瘤细胞增殖活性,可作为判断肺癌患者预后的指标之一,易被广大基层单位推广应用     

P 7IkZP i、EF Z- 1在胃癌中的表达及其相关性研究

目的：研究p27^kip1蛋白、转录因子E2F-1在胃癌中的表达及其与胃癌病理参数乏问的关系,并探讨二者相关性。方法：应用免疫组化S-P法,对90例胃癌患者的癌组织、34例癌旁正常胃黏膜进行检测,分析p27^kip1、E2F-1蛋白表达及其与胃癌病理参数之间的关系。结果：p27^kip1在正常胃组织、胃癌组织中的阳性率分别为55．9％（19／34）、31．1％（28／90）,二者差异有统计学意义（p〈0．05）。其阳性表达率与胃癌组织的浸润深度（p〈0．05）、组织学分型（p〈0．01）、分化程度（p〈0．01）、淋巴结转移（p〈0．05）均相关;E2F-1在正常胃组织、胃癌组织中的阳性率分别为17．6％（6／34）、36．7％（33／90）,二者差异有统计学意义（p〈0．05）,其阳性表达率与胃癌的组织学分型相关。而与胃癌的浸润深度（p〉0．05）、分化程度（p〉0．05）、淋巴结转移无关（p〉0．05）。结论：p27^kip1在胃癌组织中的表达明显低于在正常组织,相反,E2F-1蛋白在胃癌组织中的表达却明显增强;p27^kip1蛋白表达与胃癌的浸润深度、组织学分型、分化程度、淋巴结转移等病理参数相关;E2F-1表达与胃癌的组织学分型相关;p27^kip1、E2F-1在胃癌中的表迭呈负相关。     

Dynamic changes in p27kip1 variant expression in activated lymphocytes

The p27Kip1 cell cycle inhibitor (p27) has emerged as a critical mediator of normal cellular growth control. We report the expression of a 24 kD C-terminal variant of p27 in normal peripheral blood lymphocytes. This variant is rapidly degraded in a proteasome-dependent manner when lymphocytes are activated by interleukin-2 or by superantigen. Whereas p24 degradation is complete within 16 h of mitogen addition, full-length p27 is decreased only modestly over 72 h of mitogen exposure and is present in activated and cycling lymphocytes. Persistent p27 is present in a complex with cyclin D3 in activated lymphocytes, and is localized both in the nucleus and cytoplasm. These results indicate that lymphocytes exiting from quiescence use several mechanisms to overcome the p27Kip1-enforced cell cycle checkpoint, and that elimination of p27 is not required for cell cycle entry.     

p27kip1 overexpression promotes paclitaxel-induced apoptosis in pRb-defective SaOs-2 cells

p27kip1 is a cyclin-dependent kinase (CDK) inhibitor, which controls several cellular processes in strict collaboration with pRb. We evaluated the role of p27kip1 in paclitaxel-induced apoptosis in the pRb-defective SaOs-2 cells. Following 48 h of exposure of SaOs-2 cells to 100 nM paclitaxel, we observed an increase in p27kip1 expression caused by the decrease of the ubiquitin-proteasome activity. Such increase was not observed in SaOs-2 cells treated with the caspase inhibitors Z-VAD-FMK, suggesting that p27kip1 enhancement at 48 h is strictly related to apoptosis. Finally, we demonstrated that SaOs-2 cells transiently overexpressing the p27kip1 protein are more susceptible to paclitaxel-induced apoptosis than SaOs-2 cells transiently transfected with the empty vector. Indeed, after 48 h of paclitaxel treatment, 41.8% of SaOs-2 cells transiently transfected with a pcDNA3-p27kip1 construct were Annexin V-positive compared to 30.6% of SaOs-2 cells transfected with the empty vector (P < 0.05). In conclusion, we demonstrated that transfection of the pRb-defective SaOs-2 cells with the p27kip1 gene via plasmid increases their susceptibility to paclitaxel-induced apoptosis. The promoting effect of p27kip1 overexpression on apoptosis makes p27kip1 and proteasomal inhibitors interesting tools for therapy in patients with pRb-defective cancers.     

PP2A通过Akt/Skp2通路调控p27~(Kip1)的表达并抑制肺癌细胞的致瘤能力

蛋白磷酸酶2A(PP2A)是由36 k Da的催化亚基C(PP2Ac)和65 k Da的结构亚基A(PP2Aα/β)一起组成PP2A的核心酶,并且和各种不同的调节亚基B形成具有不同功能的PP2A全酶复合体。在细胞中PP2A发挥着重要作用,特别是在抑制肿瘤的形成当中,编码PP2Aα/β基因的突变将导致肿瘤的形成和其他疾病。当非小细胞肺癌细胞H1299中过表达PP2A-Aα时,细胞生长被抑制,细胞周期停留在G0/G1期,致瘤能力也同时被抑制。进一步研究证明当PP2A-Aα过表达时,Akt被去磷酸化失活使Skp2的表达下调,从而导致细胞周期抑制因子p27kip1的表达上调。肿瘤细胞软琼脂克隆形成实验的结果表明过表达PP2A-Aα之后H1299细胞的锚定非依赖性生长能力明显的降低,形成的克隆细胞团也较小,这些结果和裸鼠成瘤实验的结果是一致的。     

Loss of p27kip1 suppresses the myocardial senescence caused by estrogen deficiency

Estrogen deficiency accelerates the aging process and increases the risk of developing cardiovascular disease (CVD). Apoptosis is one of the important mechanisms of aging. p27^kip1 is a cyclin-dependent kinase inhibitor that can regulate cell cycle, apoptosis, and cell motility. p27^kip1 overexpression can inhibit cell cycle and increase apoptosis so it has been considered as a marker of aging. In the present study, bilateral ovariectomy (OVX) was performed as a model for menopause in wild-type (WT) and p27^kip1 knockout (KO) mice to assess the effects of p27^kip1 loss in myocardial aging caused by estrogen deficiency. We found that myocardial fibrosis and heart weight/body weight ratio of mice in the OVX group and p27^kip1 KO group were significantly increased. Echocardiography showed that the left ventricular diameter and volume of the WT OVX group increased significantly and the cardiac function decreased. However, there was no significant difference in the results of echocardiography between the two p27^kip1 KO groups. The aging and apoptosis indexes in OVX group were increased significantly, However, the indexes in p27^kip1 KO mice were decreased. The expression of antioxidant indexes in OVX group was decreased significantly and p27^kip1 KO can improve the antioxidant ability. These results provided that estrogen deficiency increased oxidative stress and apoptosis, accelerated aging of heart. p27^kip1 KO can partly delay the aging and apoptosis of heart through upregulated antioxidant enzymes.     

p27(kip1) upregulated by hnRNPC1/2 antagonizes CagA (a virulence factor of Helicobacter pylori)-mediated pathogenesis

Background and Aims: Infection by Helicobacter pylori is one of the major contributing factors of chronic active gastritis and peptic ulcer and is closely associated with the occurrence and progression of gastric cancer. CagA protein is a major virulence factor of H. pylori that interacts with SHP‐2, a true oncogene, to interfere with cellular signaling pathways; CagA also plays a crucial role in promoting the carcinogenesis of gastric epithelial cells. However, currently, the molecular mechanisms of gastric epithelial cells that antagonize CagA pathogenesis remain inconclusive. Methods: We showed that AGS gastric cancer cells transfected with CagA exhibited the inhibition of proliferation and increased activity of caspase 3/7 using two‐dimensional gel electrophoresis and secondary mass spectrometry (MS/MS). Results: It was found that the AGS gastric cancer cells stably expressing CagA displayed significantly increased the expression of 16 proteins, including hnRNPC1/2. Further analysis revealed that hnRNPC1/2 significantly boosted the expression of the p27^kip1 protein. Conclusion: Our data suggested that hnRNPC1/2 upregulates p27^kip1 expression and the subsequent suppression of cell proliferation and induction of apoptosis, thereby providing an important mechanism whereby gastric epithelial cells antagonize CagA‐mediated pathogenesis.