核糖体蛋白基因表达与肿瘤的关系

核糖体蛋白是组成核糖体的主要成分,在细胞内蛋白质生物合成中发挥重要作用。近来人们发现,核糖体具有参与DNA修复、细胞发育调控和细胞分化等核糖体外功能。并且在胃癌、结直肠癌、食管癌和肝癌等肿瘤组织中一些核糖体蛋白基因高表达,通过对肿瘤组织中核糖体蛋白基因高表达的深入研究,可以进一步阐明肿瘤发生、发展的机制,了解核糖体蛋白基因高表达在恶性肿瘤中的作用,为肿瘤的基因诊断和基因治疗开辟一个新的研究领域。     

多功能蛋白Geminin的研究进展

Geminin是一种定位于核内的多功能小分子蛋白,具有相对复杂的结构模式,在细胞增殖、胚胎发育及肿瘤发生等多方面均发挥重要作用.它通过调节细胞周期时相中的重要事件作用于细胞增殖:经多种途径参与DNA复制的调节;抑制中心体重复复制;推进G2/M期和维持正常胞质分裂等.在不同发育阶段,Geminin可作为抑制因子或是诱导因子参与胚胎发育的调节,特别是在神经形成方面.通过与同源异型盒基因或蛋白Six3及Hox等的相互作用,Geminin分别在眼睛发育及胚胎发育过程中起调节作用,并且表现出在细胞增殖与分化中协调因子的功能.近年来Geminin在肿瘤中的作用已成为研究的重点,它可作为评价肿瘤发生进程和预后的标志分子,并可望是一个新的肿瘤治疗的作用靶点.对Geminin活性的调节主要表现在转录水平和转录后水平,转录后水平的调节可能占主要地位.     

泛素连接酶FBW7的肿瘤抑制作用和机制

泛素-蛋白酶体系统是一个主要的蛋白质降解调节通路,在细胞分裂过程中发挥着重要作用,其成员在肿瘤中频繁存在着表达异常现象.FBW7又名AGO、hCDC4、FBXW7和SEL-10,是一种拥有7串联WD40重复结构域的F-box蛋白,可作为SCF型泛素连接酶（E3）复合物的底物识别亚基发挥作用.FBW7是一种肿瘤抑制蛋白,其基因在多种肿瘤包括直肠癌、胃癌、卵巢癌和白血病中存在着基因突变或缺失.FBW7可直接结合和靶向作用多种转录激活因子或原癌基因,如周期蛋白E、c-Myc、c-Jun、Notch、MCL1、KLF5 和mTOR等并对其进行泛素化修饰和随后的26S蛋白酶体降解.肿瘤抑制蛋白FBW7的研究对肿瘤发生机制的理解具有重要意义,同时也为肿瘤的诊断和治疗提供了新的靶点.本文综述了FBW7的特征、肿瘤抑制作用及机制.     

VPS35在肿瘤发生与转移中的作用及机制研究

VPS35是Retromer复合体的重要组成部分,在内吞体蛋白分选转运过程中有重要作用.最近研究表明,VPS35作为一种新的致癌基因,在多种肿瘤中高表达,调控多种因子及通路,从而影响肿瘤的发生发展和转移.本文综述了目前VPS35调控肿瘤相关因子及通路进而促进肿瘤发生与转移的最新研究进展,总结讨论了VPS35在肿瘤发生与转移中的作用机制,为将来深入研究VPS35/Retromer组分在肿瘤发生转移中的作用及机制提供借鉴与参考.     

泛素化特异性酶（USP2a）与肿瘤发生的相关分子机制

去泛素化酶USP2a是去泛素化酶家族(DUBs)的一个成员,为半胱氨酸蛋白酶,是一种重要的特异性去泛素化水解酶。USP2a具有结构和功能多样性,其结构多样化使得这些酶具有一些特异性作用靶点,特别是在基因表达调控中靶向的生理底物种类繁多。特异性蛋白泛素化水平的动态变化涉及到基因表达活化和失活的多种机制以及信号通路转导的多个环节。越来越多的文献报道了去泛素化酶相互作用网络的组成及其重要性。USP2a调节多种重要的细胞生长和分化调节因子及信号转导因子的稳定性和功能,通过USP2a的去泛素化作用以及诱导它们之间相互反应对机体进行相应调控,特别是在调控转录因子、细胞周期和细胞凋亡自噬上发挥重要作用。USP2a的过表达在体内外都表现出致癌性,其靶蛋白通过各种途径影响肿瘤发生发展。通过对人类肿瘤发生发展的相关分子机制及信号通路影响的深入研究,USP2a有望成为肿瘤治疗的新靶点。现就去泛素化酶与人类肿瘤发生发展的相关分子机制及该领域的研究进展作一综述。     

肌切蛋白的结构与功能多样性

肌切蛋白（scinderin）是一种重要的肌动蛋白结合蛋白,在哺乳动物和脊椎动物中广泛表达.肌切蛋白作为凝溶胶蛋白超家族的成员之一,通过肌动蛋白丝切割、肌动蛋白聚集等方式来控制肌动蛋白的结构.肌切蛋白生物活性具有多样性,除影响肌动蛋白丝重组外,肌切蛋白还参与细胞胞吐作用、调节细胞运动、细胞分化等细胞活动.此外,肌切蛋白在慢性炎症、凝血过程、免疫性疾病和肿瘤发生发展中也发挥了重要作用.本文对肌切蛋白的结构特点、参与调节细胞的功能和机制进行概述.     

前体mRNA剪接及剪接调节因子SR蛋白和Tra2蛋白

在高等真核生物中,前体mRNA的剪接及其调节是一个复杂的、由多因子参与的过程,它对基因的正常功能的发挥起着重要的作用,任何一种剪接调节因子的异常变化均有可能导致疾病的发生。因此,研究参与前体mRNA剪接调控的相关因子的功能及作用机制,对前体mRNA剪接机制的阐明,无疑是相当必要的。本文着重介绍了两类重要的mRNA剪接调节蛋白——SR蛋白和Tra2蛋白的研究近况,以期对前体mRNA剪接机制的研究的重要性和复杂性有更多的了解。     

WDR蛋白在肿瘤发生发展中的作用机制

WDR蛋白家族(Trp-asp repeat protein family)是含有多个保守WD基序(WD motif)的蛋白质类,广泛存在于真核生物中。近年,WDR蛋白的研究已成为细胞生物学和病理学研究的新热点。目前已知多种WDR蛋白在肿瘤细胞中异常表达,并通过调节信号转导、细胞周期、泛素化、转录和RNA加工等生物过程促使肿瘤发生。现对WDR蛋白在肿瘤发生发展中的作用机制作一综述。     

核内小体的复杂结构与多样化功能

核内小体是定位于细胞核内的无膜结构,为多蛋白-RNA复合体,通过招募相关蛋白参与基因转录、RNA剪切、表观遗传调控、肿瘤发生与抑制及抗病毒防御等多种细胞活动。明确核内小体蛋白的形成过程、功能和调控机制对研究相关疾病与病毒-宿主作用机制均具有重要意义。以下以几种核内小体蛋白为例,对核内小体的形成方式、结构与功能进行综述,并重点阐述其在抗病毒感染中的重要作用,期望为宿主抗病毒免疫机制研究提供一个新的靶标。     

RabGTPase激活蛋白结构与功能

RabGTPase激活蛋白(RabGAPs)是一类含有TBC (Tre2/Bub2/Cdc16)结构域的蛋白家族,在Rab活性调节中起着失活Rab的作用。 近年的研究表明,RabGAPs蛋白通过与特定Rab相互作用参与细胞内膜泡运输的调节。 人类RabGAPs突变涉及细胞的极性运输、糖尿病和肿瘤发生等过程,植物RabGAPs蛋白介导病毒的细胞内迁移及气孔免疫等行为。 重要的是,RabGAPs作为一个关键的调节节点,整合Rab与其他小G蛋白之间的信号进而确保囊泡正确的分选、运输及锚定到不同的胞内膜泡系统。 本文综述了RabGAPs蛋白的结构特征、生理功能、底物识别及作用机制,并对RabGAPs蛋白未来的研究方向进行了展望。     

GAIP Interacting Protein C-Terminus Regulates Autophagy and Exosome Biogenesis of Pancreatic Cancer through Metabolic Pathways

GAIP interacting protein C terminus (GIPC) is known to play an important role in a variety of physiological and disease states. In the present study, we have identified a novel role for GIPC as a master regulator of autophagy and the exocytotic pathways in cancer. We show that depletion of GIPC-induced autophagy in pancreatic cancer cells, as evident from the upregulation of the autophagy marker LC3II. We further report that GIPC regulates cellular trafficking pathways by modulating the secretion, biogenesis, and molecular composition of exosomes. We also identified the involvement of GIPC on metabolic stress pathways regulating autophagy and microvesicular shedding, and observed that GIPC status determines the loading of cellular cargo in the exosome. Furthermore, we have shown the overexpression of the drug resistance gene ABCG2 in exosomes from GIPC-depleted pancreatic cancer cells. We also demonstrated that depletion of GIPC from cancer cells sensitized them to gemcitabine treatment, an avenue that can be explored as a potential therapeutic strategy to overcome drug resistance in cancer.     

PDZ domain protein GIPC interacts with the cytoplasmic tail of melanosomal membrane protein gp75 (tyrosinase-related protein-1).

Tyrosinase and tyrosinase-related proteins (TRPs) are a family of melanosomal membrane proteins involved in mammalian pigmentation. Whereas the melanogenic functions of TRPs are localized in their amino-terminal domains that reside within the lumen of melanosomes, the sorting and targeting of these proteins to melanosomes is mediated by signals in their cytoplasmic domains. To identify proteins that interact with the cytoplasmic tail of gp75 (TRP-1), the most abundant melanosomal membrane protein, we performed yeast two-hybrid screening of a melanocyte cDNA library. Here, we show that the cytoplasmic domain of gp75 interacts with a PDZ domain-containing protein. The gp75-interacting protein is identical to GIPC, an RGS (regulator of G protein signaling)/GAIP-interacting protein, and to SEMCAP-1, a transmembrane semaphorin-binding protein. Carboxyl-terminal amino acid residues, Ser-Val-Val, of gp75 are necessary and sufficient for interaction of gp75 with the single PDZ domain in GIPC. Although endogenous and transfected GIPCs bind efficiently to transiently expressed gp75, only a small amount of GIPC is found associated with gp75 at steady state. Using a strategy to selectively synchronize the biosynthesis of endogenous gp75, we demonstrate that only newly synthesized gp75 associates with GIPC, primarily in the juxtanuclear Golgi region. Our data suggest that GIPC/SEMCAP-1 plays a role in biosynthetic sorting of proteins, specifically gp75, to melanosomes.     

Human papillomavirus type 18 E6 protein binds the cellular PDZ protein TIP-2/GIPC, which is involved in transforming growth factor beta signaling and triggers its degradation by the proteasome

Several viral proteins expressed by DNA or RNA transforming viruses have the particular property of binding via their C-terminal end to various cellular proteins with PDZ domains. This study is focused on the PDZ protein TIP-2/GIPC, which was originally identified in two-hybrid screens performed with two different baits: the human T-cell leukemia virus type 1 Tax oncoprotein and the regulator of G signaling RGS-GAIP. Further studies have shown that TIP-2/GIPC is also able to associate with the cytoplasmic domains of various transmembrane proteins. In this report we show that TIP-2/GIPC interacts with the E6 protein of human papillomavirus type 18 (HPV-18). This event triggers polyubiquitination and proteasome-mediated degradation of the cellular protein. In agreement with this observation, silencing of E6 by RNA interference in HeLa cells causes an increase in the intracellular TIP-2/GIPC level. This PDZ protein has been previously found to be involved in transforming growth factor beta (TGF-beta) signaling by favoring expression of the TGF-beta type III receptor at the cell membrane. In line with this activity of TIP-2/GIPC, we observed that depletion of this protein in HeLa cells hampers induction of the Id3 gene by TGF-beta treatment and also diminishes the antiproliferative effect of this cytokine. Conversely, silencing of E6 increases the expression of Id3 and blocks proliferation of HeLa cells. These results support the notion that HPV-18 E6 renders cells less sensitive to the cytostatic effect of TGF-beta by lowering the intracellular amount of TIP-2/GIPC.     

Regulation of mitochondrial fission by GIPC-mediated Drp1 retrograde transport

Dynamin-related protein 1 (Drp1) is a key regulator of mitochondrial fission, a large cytoplasmic GTPase recruited to the mitochondrial surface via transmembrane adaptors to initiate scission. While Brownian motion likely accounts for the local interactions between Drp1 and the mitochondrial adaptors, how this essential enzyme is targeted from more distal regions like the cell periphery remains unknown. Based on proteomic interactome screening and cell-based studies, we report that GAIP/RGS19-interacting protein (GIPC) mediates the actin-based retrograde transport of Drp1 toward the perinuclear mitochondria to enhance fission. Drp1 interacts with GIPC through its atypical C-terminal PDZ-binding motif. Loss of this interaction abrogates Drp1 retrograde transport resulting in cytoplasmic mislocalization and reduced fission despite retaining normal intrinsic GTPase activity. Functionally, we demonstrate that GIPC potentiates the Drp1-driven proliferative and migratory capacity in cancer cells. Together, these findings establish a direct molecular link between altered GIPC expression and Drp1 function in cancer progression and metabolic disorders.     

GIPC and GAIP form a complex with TrkA: a putative link between G protein and receptor tyrosine kinase pathways

NGF initiates the majority of its neurotrophic effects by promoting the activation of the tyrosine kinase receptor TrkA. Here we describe a novel interaction between TrkA and GIPC, a PDZ domain protein. GIPC binds to the juxtamembrane region of TrkA through its PDZ domain. The PDZ domain of GIPC also interacts with GAIP, an RGS (regulators of G protein signaling) protein. GIPC and GAIP are components of a G protein-coupled signaling complex thought to be involved in vesicular trafficking. In transfected HEK 293T cells GIPC, GAIP, and TrkA form a coprecipitable protein complex. Both TrkA and GAIP bind to the PDZ domain of GIPC, but their binding sites within the PDZ domain are different. The association of endogenous GIPC with the TrkA receptor was confirmed by coimmunoprecipitation in PC12 (615) cells stably expressing TrkA. By immunofluorescence GIPC colocalizes with phosphorylated TrkA receptors in retrograde transport vesicles located in the neurites and cell bodies of differentiated PC12 (615) cells. These results suggest that GIPC, like other PDZ domain proteins, serves to cluster transmembrane receptors with signaling molecules. When GIPC is overexpressed in PC12 (615) cells, NGF-induced phosphorylation of mitogen-activated protein (MAP) kinase (Erk1/2) decreases; however, there is no effect on phosphorylation of Akt, phospholipase C-gamma1, or Shc. The association of TrkA receptors with GIPC and GAIP plus the inhibition of MAP kinase by GIPC suggests that GIPC may provide a link between TrkA and G protein signaling pathways.     

Interactions between GIPC-APPL and GIPC-TRP1 regulate melanosomal protein trafficking and melanogenesis in human melanocytes

By virtue of the presence of multiple protein–protein interaction and signaling domains, PDZ proteins play important roles in assembling protein complexes that participate in diverse cell biological processes. GIPC is a versatile PDZ protein that binds a variety of target proteins in different cell types. In previous studies we showed that, in epidermal melanocytes, GIPC interacts with newly synthesized melanosomal protein TRP1 in the Golgi region and proposed that this interaction may facilitate intracellular trafficking of TRP1. However, since GIPC contains a single PDZ domain and no other known protein interaction motifs, it is not known how GIPC–TRP1 interaction affects melanosome biogenesis and/or melanin pigmentation. Here, we show that in human primary melanocytes GIPC interacts with AKT-binding protein APPL (adaptor protein containing pleckstrin homology, leucine zipper and phosphotyrosine binding domains), which readily co-precipitates with newly synthesized TRP1. Knockdown of either GIPC or APPL inhibits melanogenesis by decreasing tyrosinase protein levels and enzyme activity. In melanocytes, APPL exists in a complex with GIPC and phospho-AKT. Inhibition of AKT phosphorylation using a PI3-kinase inhibitor abolishes this interaction and results in retardation TRP1 in the Golgi. These data suggest that interactions between TRP1–GIPC and GIPC–APPL–AKT provide a potential link between melanogenesis and PI3 kinase signaling.     

TRP1 interacting PDZ-domain protein GIPC forms oligomers and is localized to intracellular vesicles in human melanocytes

PDZ proteins coordinate assembly of protein complexes that participate in diverse biological processes. GIPC is a multifunctional PDZ protein that interacts with several soluble and membrane proteins. Unlike most PDZ proteins, GIPC contains single PDZ domain and the mechanisms by which GIPC mediates its actions remain unclear. We investigated the possibility that in lieu of multiple PDZ domains, GIPC forms multimers. Here, we demonstrate that GIPC can bind to itself and that the PDZ domain is involved in GIPC-GIPC interaction. Gel filtration, sucrose gradient centrifugation and chemical cross-linking showed that whereas bulk of cytosolic GIPC was present as monomer, oligomers with an estimated molecular mass corresponding to GIPC homotrimer were readily detectable in the membrane fraction. Modeling of GIPC PDZ domain showed feasibility of trimerization. Immunogold electron microscopy showed that GIPC is present in clusters near vesicles. Our data suggest that oligomers of GIPC mediate its functions in melanocytes.     

GLUT1CBP(TIP2/GIPC1) interactions with GLUT1 and myosin VI: evidence supporting an adapter function for GLUT1CBP

We identified a novel interaction between myosin VI and the GLUT1 transporter binding protein GLUT1CBP(GIPC1) and first proposed that as an adapter molecule it might function to couple vesicle-bound proteins to myosin VI movement. This study refines the model by identifying two myosin VI binding domains in the GIPC1 C terminus, assigning respective oligomerization and myosin VI binding functions to separate N- and C-terminal domains, and defining a central region in the myosin VI tail that binds GIPC1. Data further supporting the model demonstrate that 1) myosin VI and GIPC1 interactions do not require a mediating protein; 2) the myosin VI binding domain in GIPC1 is necessary for intracellular interactions of GIPC1 with myosin VI and recruitment of overexpressed myosin VI to membrane structures, but not for the association of GIPC1 with such structures; 3) GIPC1/myosin VI complexes coordinately move within cellular extensions of the cell in an actin-dependent and microtubule-independent manner; and 4) blocking either GIPC1 interactions with myosin VI or GLUT1 interactions with GIPC1 disrupts normal GLUT1 trafficking in polarized epithelial cells, leading to a reduction in the level of GLUT1 in the plasma membrane and concomitant accumulation in internal membrane structures.     

Synectin, syndecan-4 cytoplasmic domain binding PDZ protein, inhibits cell migration

Syndecan-4, a member of the syndecan gene family of proteoglycans, is an important regulator of bFGF signaling. In particular, bFGF-dependent regulation of cell growth and migration has been linked to syndecan-4 cytoplasmic domain-mediated interactions. Screening of a yeast two-hybrid library with a cytoplasmic domain of rat syndecan-4 identified a novel binding partner, here termed synectin. Synectin is highly homologous to semaphorin F binding protein semcap1, glucose 1 transporter binding protein glut1cbp, and RGS-GAIP/neuropilin-1 binding protein GIPC. Overexpression of synectin in ECV304 cells in culture led to a dose-dependent inhibition of migration while not affecting cell adhesion or growth rate. We conclude that synectin is involved in syndecan-4-dependent interactions and may play a role in the assembly of syndecan-4 signaling complex.     

5T4 Interacts with TIP-2/GIPC, a PDZ Protein, with Implications for Metastasis

Overexpression of the 5T4 transmembrane glycoprotein can have marked effects on both the actin cytoskeleton and cell migration. Using a yeast two-hybrid approach, we describe a novel interaction between 5T4 and TIP-2/GIPC, a cytoplasmic interacting protein containing a PDZ domain. The cytoplasmic tail of 5T4 contains a class I PDZ-binding motif (Ser-Asp-Val) and we demonstrate that this region, in particular the terminal valine, is required for 5T4 interaction with TIP-2/GIPC. HeLa cells expressing hemagglutinin-tagged TIP-2/GIPC (HA-TIP-2/GIPC) have an altered distribution of endogenous 5T4, which colocalizes with HA-TIP-2/GIPC, thus supporting an interaction. Furthermore, TIP-2/GIPC can be coimmunoprecipitated with 5T4 from HeLa cell lysates. Identification of the 5T4 and TIP-2/GIPC interaction provides the first link between 5T4 and the actin cytoskeleton. Since other proteins, like 5T4, associate with TIP-2/GIPC and are linked with cancer, we explore the possibility that TIP-2/GIPC may be a common factor involved in the cancer process.