p73基因研究进展

新近发现的p53家族成员－p53基因,其结构和功能均与p53有相似之处。p53蛋白可与多种病毒,胞内信号分子,p53蛋白及其他调节蛋白作用,参与粒细胞分化及T细胞凋亡等多种生理过程;还不清楚p53介否作为一种抑癌基因。     

p63亚型及其与疾病的相关性

p63足p53家族成员的核转录因子,根据N端及C端的不同,已经发现TAp630α、TAp63β、rap63y、ANp630α、△Np63β、△Np63β、△Np63δ、△Np63δ种亚型。p63的表达受到多种转录因子的调控,其mRNA的稳定性由RNPCI调节,蛋白的稳定性主要由HECT家族成员Itch／AIP4、WWPI调节。p63在上皮细胞分化、组织发育过程中起着关键性作用,因此,p63基因突变可以导致外胚层发育不良的相关疾病,同时,p63在肿瘤的形成和转移的过程中具有重要的调控作用。     

miR-34家族——-肿瘤抑制蛋白p53高度相关microRNA

若干微小RNA(microRNA, miRNA)与肿瘤抑制蛋白p53高度相关, 其中miR-34家族最具代表性。一方面p53可通过对miR-34家族的调控实现对多个原癌基因如Bcl-2、c-myc以及细胞因子如cyclinE2、cyclinD1和c-Met的抑制, 进而发挥抑癌作用; 另一方面miR-34家族也可以通过抑制沉默信息调节子SIRTI来进一步增强p53的活性。p53与miR-34家族之间形成的正反馈调节网络对抑制肿瘤的发生发展及恶化均起着重要的作用。文章对p53高度相关的miR-34家族在肿瘤发生发展及治疗的最新进展作一论述。     

p21活化激酶的生物学活性及其与肿瘤的关系

p21活化激酶(p21-activatedkinase,PAK),为一类进化上保守的丝氨酸/苏氨酸蛋白激酶。PAK在许多组织中广泛表达,作为小G蛋白Rho家族Cdc42和Rac1的下游靶蛋白,可以被生长因子及其他胞外信号通过GTP酶依赖的信号通路或非GTP酶依赖的信号通路活化,发挥多种生物学效应。PAK作为一种重要的生物学调节因子,在哺乳动物一系列细胞功能中具有重要作用,如:细胞运动、细胞生存、细胞周期、血管生成、基因转录调节及癌细胞的侵袭转移。通过对PAK家族成员信号转导机制的研究,为癌症治疗提供分子靶标。     

心肌特异表达的肌小节相关激酶基因p93的克隆与鉴定

心肌收缩受到由蛋白质因子构成的信号转导通路的调控 ,但确切机制尚未完全明了。从人心脏cDNA文库中克隆到心肌特异表达的可能参与信号转导调控的新基因 ,命名为p93基因。该基因定位于 1p31.1,属于MAP KKKs家族的相近亚家族。Northern印迹及含 76种组织的点杂交显示了p93仅在心肌组织中表达 ;免疫组化表明它主要定位于成人与胎儿的心肌细胞核 ,胞液次之 ;体外激酶活性实验证明野生型p93是一个可以进行自我磷酸化的功能性激酶分子 ;以该基因C端为诱饵质粒的酵母双杂交筛选表明 ,p93主要与心肌肌钙蛋白I(cTnI)等与收缩有关的肌小节蛋白发生相互作用 ,并以免疫共沉淀实验得到了验证。推测p93可能通过激酶信号转导通路的方式参与对肌小节收缩蛋白的调节。     

Smyd1蛋白的研究进展

Smyd1是组蛋白甲基转移酶,在心肌和骨骼肌中特异表达,是调节心肌和骨骼肌发育的关键因子。本文简要综述了Smyd1蛋白的结构组成、作用机理及其在心肌和骨骼肌生长发育中的作用,为开展进一步研究提供参考。     

肿瘤细胞中存活蛋白与p53的相互作用

存活蛋白(survivin)作为凋亡抑制蛋白(IAP)家族的最小成员,在肿瘤组织中高表达,且具有严格的细胞周期依赖性,而p53作为细胞周期中的负调节因子,参与了细胞周期调控和细胞凋亡等重要的生物学功能。最近研究表明,存活蛋白与p53的相互作用在肿瘤的发生发展中具有重要作用。该文将从细胞周期与细胞凋亡的角度对存活蛋白/p53通路在肿瘤中的研究进展进行阐明。     

p38γ/SAPK3信号传导通路及其生物学功能

p38γ（又称为SAPK3、ERK6）是MAPK家族的一个新成员,其组织分布具有高度特异性,在骨骼肌中大量表达。p38γ／SAPK3信号传导通路可引起多种细胞生物学反应,如细胞增殖、分化、转化及凋亡等,其级联途径的上游分子及激活方式、下游分子及效应方式又与MAPK家族其他成员显著不同。本文重点讨论近年来国内外对p38γ／SAPK3的结构、信号通路组成及其生物学功能的研究进展。     

鼻咽癌CT 表现与p53 、p16 蛋白异常表达关系的研究

目的：研究p53、p16蛋白表达与鼻咽癌Cr表现的关系。方法：经病理证实鼻咽癌50例,全部病例做鼻咽轴位平扫,部分病例同时做冠状扫描。应用免疫组化SABC法检测所有病例中的p53、p16蛋白的表达。结果：鼻咽癌及鼻咽粘膜慢性炎症中p53蛋白表达率分别为60％和10％,p16蛋白表达率分别为32％和85％,p53、p16表达在两者间的差异有极显著意义（P〈0．005）。p53蛋白表达与鼻咽癌分化程度及Cr表现为副鼻窦受累,颅底骨质破坏相关（P〈0．05）。p16蛋白表达与鼻咽癌预后及Cr表现为颈部淋巴结转移相关（P〈0．05）。p53与p16有相关性（P〈0．005）。结论：p53、p16在鼻咽发生、发展中起重要作用,p53蛋白表达与鼻咽癌分化程度、浸润深度、颅底侵犯有一定相关性,p16蛋白表达与鼻咽癌颈部淋巴结转移和预后有一定相关性,p53,p16可作为评价鼻咽癌CT表现恶性度及预后的指标。     

SCF泛素连接酶靶蛋白识别组分FBW7

FBW7（F-box and WD repeat domain-containing7）是F-box蛋白家族成员,为SCF（SKP1-CUL1-F-box）型泛素连接酶的靶蛋白识别组分。FBW7通过靶降解周期蛋白E、Myc、Jun等多种癌蛋白,对细胞周期进程、细胞生长、分化起重要调控作用。在多种人类肿瘤中已发现FBW7突变,FBW7功能缺失会引起染色体不稳定及肿瘤发生,表明FBW7是一种肿瘤抑制因子。在FBW7缺失所致的肿瘤发生过程中,周期蛋白E、Myc等靶蛋白活性升高、p53功能缺失有重要作用。     

Cloning and characterisation of Ifi206: a new murine HIN-200 family member

HIN-200 proteins are interferon-inducible proteins capable of regulating cell growth, senescence, differentiation and death. Using a combination of in silico analysis of NCBI EST databases and screening of murine C57BL/6 cDNA libraries we isolated novel murine HIN-200 cDNAs designated Ifi206S and Ifi206L encoding two putative mRNA splice variants. The p206S and p206L protein isoforms have a modular domain structure consisting of an N-terminal PAAD/DAPIN/Pyrin domain, a region rich in serine, threonine and proline residues and a C-terminal 200 B domain characteristic of other HIN-200 proteins. Ifi206 mRNA was detected only in the spleen and lung of BALB/c and C57BL/6 mice and expression was up-regulated by both types I and II IFN subtypes. p206 protein was predominantly expressed in the cytoplasm and addition of LMB, a CRM1 dependent nuclear export inhibitor, caused p206 to accumulate in the nucleus. Unlike other human and mouse HIN-200 proteins that contain only a single 200 amino acid domain, overexpression of p206 impaired the clonogenic growth of tumour cell lines. Thus, p206 represents the newest HIN-200 family member discovered. It has distinct and restricted pattern of expression however maintains many of the hallmarks of HIN-200 proteins including the presence of a characteristic 200 X domain, induction by interferon and an ability to suppress tumour cell growth.     

Characterization of a brain-specific Rho GTPase-activating protein,p200RhoGAP

The Rho GTPase-activating proteins (RhoGAPs) are a family of multifunctional molecules that transduce diverse intracellular signals by regulating Rho GTPase activities. A novel RhoGAP family member, p200RhoGAP, is cloned in human and mouse. The murine p200RhoGAP shares 86% sequence identity with the human homolog. In addition to a conserved RhoGAP domain at the N terminus, multiple proline-rich motifs are found in the C-terminal region of the molecules. Northern blot analysis revealed a brain-specific expression pattern of p200RhoGAP. The RhoGAP domain of p200RhoGAP stimulated the GTPase activities of Rac1 and RhoA in vitro and in vivo, and the conserved catalytic arginine residue (Arg-58) contributed to the GAP activity. Expression of the RhoGAP domain of p200RhoGAP in Swiss 3T3 fibroblasts inhibited actin stress fiber formation stimulated by lysophosphatidic acid and platelet-derived growth factor-induced membrane ruffling but not Bradykinin-induced filopodia formation. Endogenous p200RhoGAP was localized to cortical actin in naive N1E-115 neuroblastoma cells and to the edges of extended neurites of differentiated N1E-115 cells. Transient expression of the RhoGAP domain and the full-length molecule, but not the catalytic arginine mutants, readily induced a differentiation phenotype in N1E-115 cells. Finally, p200RhoGAP was capable of binding to the Src homology 3 domains of Src, Crk, and phospholipase Cgamma in vitro and became tyrosine-phosphorylated upon association with activated Src in cells. These results suggest that p200RhoGAP is involved in the regulation of neurite outgrowth by exerting its RhoGAP activity and that its cellular activity may be regulated through interaction with Src-like tyrosine kinases.     

Temporal and spatial assembly of lipid droplet-associated proteins in 3T3-L1 preadipocytes

This study aimed to investigate the relationship between newly formed lipid droplets and lipid droplet surface proteins, including perilipin, adipose differentiation related protein (ADRP), and p200 kDa protein (p200) in 3T3-L1 preadipocytes, during lipogenesis. Sterol ester was used to induce nascent lipid droplets in 3T3-L1 preadipocytes and the sequence of lipids and lipid droplet surface proteins was studied using a combination of immunohistochemistry and Nile red staining/Oil red O. We demonstrated that, although most growing lipid droplets appeared to have a lipid core surrounded by a fluorescent rim of ADRP, perilipin, and p200, tiny protein aggregates of ADRP, perilipin, or p200 could also be found to occur in the absence of lipid accumulation. In addition, ADRP associated with nascent lipid droplets prior to that of perilipin or p200. We provide evidence that lipid droplet surface proteins, especially ADRP and perilipin, are important in serving as a nucleation center for the assembly of lipid to form nascent lipid droplets.     

Comparative analysis of p21 proteins from various cell types by two-dimensional gel electrophoresis

The products of the ras gene family are related proteins at a molecular weight of 21 kDa, designated p21. In the present study we used two-dimensional gel electrophoresis to compare p21 proteins from five different normal and malignant cell lines. Using a known protein (3H-labeled translation initiation factor [eIF-4D]) as a standard internal marker for isoelectric point (pI), we show that p21 proteins from various cells differ only slightly in molecular weight (21-24 kDa) but express a wide variety in charge (pI 4.8 to 7) that could only be detected by the use of two-dimensional gel electrophoresis. p21 in NIH/3T3 cells was expressed as a single protein, which migrated at 21 kDa and pI 5.1. This peptide, which is probably the product of the normal cellular ras gene, was also detected in normal human lymphocytes. The synthesis of this peptide was not elevated in the transformed cells. However, transformation of NIH/3T3 fibroblasts and of human leukocytes was found to be associated with expression of qualitatively different forms of p21 peptides. Four additional p21-associated peptides of identical molecular weight (23 kDa), but multiple charge forms, were detected selectively in Kirsten murine sarcoma virus-transformed NIH/3T3 cells. Transformation of cells with Harvey murine sarcoma virus was found to be associated with prominent expression of two major pairs of p21-associated proteins, one at 21 kDa (pI, 5.2 and 5.3) and the other at 23 kDa (pI, 5.1 and 5.2). In HL-60 leukemic cells there was an additional, more acidic form (pI 5.0) of p21, which appeared to be absent or reduced in normal human lymphocytes. These results indicate that p21 from viral origin or cellular origin might be expressed in the cells in multiple charge forms. The capability to distinguish multiple forms of p21 and slight charge modifications associated with malignancy should call for the use of 2-D gel electrophoresis as an important tool in future studies involving p21 proteins.     

The cytoplasmic filaments of the nuclear pore complex are dispensable for selective nuclear protein import

Oxysterol binding proteins (OSBPs) comprise a large conserved family of proteins in eukaryotes. Their ubiquity notwithstanding, the functional activities of these proteins remain unknown. Kes1p, one of seven members of the yeast OSBP family, negatively regulates Golgi complex secretory functions that are dependent on the action of the major yeast phosphatidylinositol/phosphatidylcholine Sec14p. We now demonstrate that Kes1p is a peripheral membrane protein of the yeast Golgi complex, that localization to the Golgi complex is required for Kes1p function in vivo, and that targeting of Kes1p to the Golgi complex requires binding to a phosphoinositide pool generated via the action of the Pik1p, but not the Stt4p, PtdIns 4-kinase. Localization of Kes1p to yeast Golgi region also requires function of a conserved motif found in all members of the OSBP family. Finally, we present evidence to suggest that Kes1p may regulate adenosine diphosphate-ribosylation factor (ARF) function in yeast, and that it may be through altered regulation of ARF that Kes1p interfaces with Sec14p in controlling Golgi region secretory function.     

p63 and p73 expression in extrahepatic bile duct carcinoma and their clinical significance

p53 plays a pivotal role in the prevention of human tumor formation. p73 and p63 are new members of the p53 tumor suppressor family, which are becoming increasingly recognized as important players in human tumorigenesis. However, the roles of these proteins are not well elucidated in extrahepatic bile duct (EBD) carcinoma. We examined expressions of the p63 and p73 genes and proteins in normal biliary epithelia, biliary dysplasias, and EBD carcinomas using immunohistochemistry and RT-PCR analysis. p63 and p73 proteins were overexpressed in 26.3 and 41.0% of EBD carcinomas, respectively. p63 protein expression was more frequent in tumors with vascular invasion (P = 0.002) and distal location (P = 0.04), while p73 expression was more common in cancers with deeper tumor invasion (P = 0.04). Patients with tumors co-expressing both p63 and p73 were found to have a significantly worse overall survival rate compared to those with either p63 or p73 expression (P < 0.05) as determined in univariate and multivariate analyses. Our results strongly imply that the p53 family members have different functions in EBD carcinomas. Our data also indicate that interactions between p63 and p73 play an important role in tumorigenesis of EBD carcinoma.     

Biochemical and Functional Evidence of p53 Homology Is Inconsistent with Molecular Phylogenetics for Distant Sequences

The tumor suppressor p53 is mutated in ～50% of all human cancer cases worldwide. It is commonly assumed that the phylogenetic history of this important tumor suppressor has been thoroughly studied; however, few detailed studies of the entire extended p53 protein family have been reported, and none comprehensively and simultaneously consider functional, molecular, and phylogenetic data. Herein we examine a diverse collection of reported p53-like protein sequences, including representatives from the arthropods, nematodes, and protists, with the goal of answering several important questions. First, what evidence supports these highly divergent proteins being true homologues to the p53 family? Second, is the inferred overall family phylogeny concordant with known structures and functions? Third, does the extended p53 family possess recognizable conserved sites outside of the within-chordate, highly-conserved DNA-binding domain? Our study shows that the biochemical and functional evidence of p53 homology for nematodes, arthropods, and protists is inconsistent with their implied phylogenetic relationship within the overall family. Although these divergent sequences are always reported as functionally similar to human p53, our results confirm and extend the hypothesis that p63 is a far more appropriate protein for comparison. Within these divergent sequences, we find minimal conservation within the DNA-binding domain, and no conservation elsewhere. Taken together, our findings suggest that these sequences are not bona fide homologues of the extended p53 family and provide baseline criteria for the future identification and characterization of distant p53-family homologues.