凝溶胶蛋白与创伤后炎症反应

凝溶胶蛋白(gelsolin,GSN)是机体内重要的肌动蛋白结合蛋白,对肌动蛋白的聚合/解聚具有重要调节作用。其生理效应不仅在于维持细胞结构稳定,而且参与多种细胞活动的调节过程,是一种重要的细胞功能调节蛋白。血浆型GSN是血浆肌动蛋白清除系统主要成员之一,对维持内环境稳定非常重要。严重创伤后血浆中GSN水平显著而持续降低,且与患者预后密切相关。本文综述GSN与创伤后炎症反应的关系。     

凝溶胶蛋白对植物微丝的调节作用及在花粉中的定位

以植物花粉为实验材料, 研究了来源于动物的凝溶胶蛋白对植物肌动蛋白丝的作用及凝溶胶蛋白在植物细胞中的定位. 利用离心沉淀丝状肌动蛋白及电子显微镜负染的实验结果显示, 花粉纯化肌动蛋白丝及粗提液中肌动蛋白丝可被凝溶胶蛋白剪切, 而且这种剪切作用依赖于Ca²⁺. 另外, 利用免疫沉淀测定凝溶胶蛋白与花粉肌动蛋白单体结合的实验表明, 当溶液中有Ca²⁺. 存在时, 花粉肌动蛋白与凝溶胶蛋白的摩尔比值约为2.0 ± 0.21; 用EGTA去除Ca²⁺. 后, 该比值有所降低, 减至1.2 ± 0.23; 而加入PIP2后, 这种结合比值又降至0.8 ± 0.10, 表明植物肌动蛋白与凝溶胶蛋白的结合有类似于动物肌动蛋白的特性, 受到Ca²⁺. 和PIP2的调节. 花粉中凝溶胶蛋白的免疫鉴定及免疫荧光定位实验结果表明, 花粉中存在凝溶胶蛋白, 在未萌发的花粉粒中凝溶胶蛋白主要集中在萌发沟处, 而在萌发2 h的花粉管中, 花粉管胞质内均可看到荧光分布, 但花粉管顶端荧光较强, 推测凝溶胶蛋白可能参与花粉的萌发和花粉管的生长.     

凝溶胶蛋白治疗阿尔茨海默症的研究进展

阿尔茨海默症(Alzheimer’s disease,AD)的病理学特征之一是患者脑内存在以β-淀粉样肽(Aβ)为主要成分的老年斑。大量的实验证据表明,以Aβ为靶目标,清除老年斑有助于提高患者的认知能力,是防治AD的一个重要研究方向。凝溶胶蛋白在细胞骨架结构重排和细胞运动等过程中都发挥重要作用。目前多个小组的研究成果显示,凝溶胶蛋白与AD的发生、发展密切相关。凝溶胶蛋白能够抑制Aβ积聚形成纤维,也能够引发已形成的Aβ纤维发生解聚。更重要的是,凝溶胶蛋白能够清除转基因AD模型小鼠脑内的老年斑和降低Aβ的水平。未来凝溶胶蛋白有可能被应用于AD的预防和治疗。     

凝溶胶蛋白的结构与功能

凝溶胶蛋白（gelsolin）是凝溶胶蛋白超家族的成员之一,是一种重要的肌动蛋白结合蛋白,其通过切断、封端肌动蛋白丝,或使肌动蛋白聚集成核等方式来控制肌动蛋白的结构.凝溶胶蛋白除了在重组肌动蛋白丝中发挥作用以外,还在细胞运动、控制细胞程序性死亡等细胞活动中发挥重要的作用.此外,肿瘤细胞中凝溶胶蛋白的表达量也发生变化.凝溶胶蛋白的变异还是某些遗传疾病的基础.最近的研究发现,凝溶胶蛋白可以作为转录辅激活蛋白,促进雄激素受体的转录活性.本文对凝溶胶蛋白的结构特点、参与调节细胞的功能和机制及其研究现状进行概述.     

凝溶胶蛋白基因的生物学功能及其应用研究进展

凝溶胶蛋白(gelsolin,GSN)是Gelsolin/Villin超家族的核心成员,是一种多功能的钙依赖性肌动蛋白结合蛋白,在细胞中Ca^2+和PIP2等多因素的调控下,对细胞凋亡、吞噬功能、肌动蛋白微丝切割、细胞信号转导等方面起着重要的作用。近年来,凝溶胶蛋白还被频繁用于相关疾病的预防、诊断与治疗,但其在调控细胞凋亡、炎症等病理生理中的作用机制还存在些许争议。本研究综述了凝溶胶蛋白的结构特点、生物学功能以及对疾病的诊断和治疗,旨在了解凝溶胶蛋白在生物医学及动物科学等领域的应用以及未来凝溶胶蛋白的发展前景。     

凝溶蛋白对骨骼肌天然细肌丝的作用

凝溶蛋白是Ｆ－肌动蛋白丝的钙依赖性切割性蛋白质,经过焦磷酸溶液选择性抽提和微酸性介质的有效分离,可以得到纯度较高的天然细肌丝。在Ｃａ＾２＋存在时,凝溶蛋白可以切割天然细肌丝。但是,凝溶蛋白对天然细肌丝的作用时程与其对Ｆ－肌动蛋白丝的作用有着显差异,提示细肌丝中的非肌动蛋白蛋白质可能影响了凝溶蛋白对天然细肌丝的结合或切割速率。     

钙卫蛋白与炎症相关疾病

炎症是机体非常重要的病理过程,包括损伤、抗损伤和修复等一系列步骤,是由许多细胞和物质共同参与构成的复杂反应,但这种保护机制在过于激烈或持久时也会造成伤害或疾病.由S100钙结合蛋白家族成员S100A8和S100A9聚合而成的钙卫蛋白已被证明在感染性疾病、免疫性疾病、代谢性疾病、退行性疾病等相关炎症进程中发挥了不容忽视的...     

凝溶蛋白对骨骼肌天然细肌丝的作用

凝溶蛋白是Ｆ－肌动蛋白丝的钙依赖性切割性蛋白质．经过焦磷酸溶液选择性抽提和微酸性介质的有效分离,可以得到纯度较高的天然细肌丝．在Ｃａ２＋存在时,凝溶蛋白可以切割天然细肌丝．但是,凝溶蛋白对天然细肌丝的作用时程与其对Ｆ－肌动蛋白丝的作用有着显著差异,提示细肌丝中的非肌动蛋白蛋白质可能影响了凝溶蛋白对天然细肌丝的结合或者切割速率．     

凝溶胶蛋白及其生物医学作用

gelsolin(凝溶胶蛋白)有胞浆和血清二型,分别存在于哺乳动物各类细胞和血清中。该蛋白的基本生物功能是以钙依赖的方式通过切断、封端肌动蛋白丝,或使肌动蛋白聚集成核等方式控制肌动蛋白的结构。大量动物实验和临床研究均表明,gelsolin的结构、功能及调节与烧伤和急性挫伤的诊断与治疗,以及某些炎症、肿瘤和淀粉样变等多种疾病的病理过程密切相关。作为一种急症治疗药,该蛋白的工程化产品已在美国进行Ⅱ期临床实验。最近发现正常细胞经电离辐射后,gelsolin的表达水平发生显著改变,其在辐射效应中的作用和意义值得关注。     

细胞骨架蛋白调节囊泡转运及其与神经疾病的关系

细胞内囊泡转运依赖于细胞骨架系统,细胞骨架为囊泡转运提供了轨道,而细胞骨架表面的马达蛋白则为其提供了动力。近年来,随着活细胞成像技术以及相关的生化、药理实验方法的不断进步,人们对囊泡转运的分子机制有了更加深入的认识。越来越多的实验结果表明,细胞骨架蛋白对囊泡转运有着重要的调节作用。囊泡转运的紊乱与多种神经疾病相关。囊泡转运分子调控机制的研究,将为多种神经疾病的治疗提供新的思路。     

早期脓毒血症患者Gelsolin 与HS-1 蛋白检测及其意义

要目的：探讨脓毒血症患者血小板骨架蛋白Gelsolin和造血系细胞特异性蛋白(HS-1)及其和凝血功能的关系。方法：纳入脓毒 血症患者30 例和对照组健康人群30 例,用双抗体夹心法测定血浆中血小板骨架蛋白,用酶联免疫法测定血清中HS-1 蛋白含 量,采用免疫荧光观察血小板Gelsolin 蛋白的表达,分析Gelsolin、HS-1、血小板计数和凝血功能(PT、APTT)之间的关系。结果：对 照组Gelsolin 主要位于血小板胞浆内,观察组包浆内外及间质内均可见。观察组血小板骨架蛋白Gelsolin、HS-1 水平明显高于对 照组,差异均存在统计学意义(P<0.05)。观察组血小板计数、PT、APTT 水平均低于对照组,差异存在统计学意义(P <0.05)。Galsolin 和血小板计数呈负相关关系,相关系数r = -0.76 (P <0.05),HS-1和血小板计数间呈负相关关系相关系数r = - 0.69 (P<0.05)。结论： 早期脓毒血症患者血小板骨架蛋白Gelsolin 和HS-1表达水平明显升高,与脓毒血症患者血小板大量破坏有关。     

Isolation of a Ca2+-Dependent Actin-Fragmenting Protein from Brain, Spinal Cord, and Cultured Neurones

Extracts of ox spinal cord and chicken brain were fractionated by ion-exchange chromatography and assayed for their ability to reduce the viscosity of muscle F-actin solutions. Two distinct peaks of activity were obtained, one of which was further purified by affinity chromatography on a DNAase-actin Sepharose column. Following molecular exclusion chromatography, the actin component appeared as a complex of 1 molecule of a protein with molecular weight 90,000 and 2 molecules of actin (42,000). This tightly bound complex was resistant to most methods of protein separation, but was resolvable into its component proteins by sodium dodecyl sulphate acrylamide gel electrophoresis. The protein of molecular weight 90,000 could be eluted from such a gel in a fully active form. The activity of the protein from ox spinal cord was closely similar to that of gelsolin, an actin-fragmenting protein originally isolated from rabbit lung macrophages. Like gelsolin, the protein from ox spinal cord produced fragmentation of muscle F-actin filaments at Ca2+ concentrations greater than 10(-7) M, and had a nucleating effect on the polymerisation of muscle actin; the latter was measured most easily by the enhancement of fluorescence of muscle actin conjugated to N-(1-pyrenyl)iodoacetamide. Nucleation was more effective in the presence of Ca2+, but also occurred in its absence, and the same was true of complex formation between the 90,000 protein and muscle G-actin. On the basis of its actin-fragmenting activity, we estimate that the 90,000 molecular weight protein constitutes 0.2% of the protein initially extracted from ox spinal cord. A very similar protein, indistinguishable in its action on actin but containing variable amounts of a protein of molecular weight 85,000 as well as 90,000, was isolated from chicken brain. A similar protein was also detected in pure cultures of sympathetic neurones by enrichment on a DNAase-actin affinity column and by immune blotting and by immunofluorescence. We conclude that a protein similar, if not identical to macrophage gelsolin is present in neurones and that it probably plays a part in the actin-based movements of these cells.     

A Novel Gelsolin Isoform Expressed by Oligodendrocytes in the Central Nervous System

Abstract: Two isoforms of the Ca²⁺-sensitive, actin-binding protein gelsolin have been identified thus far; one is an intracellular protein, cytoplasmic gelsolin, and the other is a secretory protein called plasma gelsolin. Gelsolin expression in the mammalian CNS appears to be localized mainly to oligodendrocytes where it is presumed that the cytoplasmic isoform predominates. Here, we show that oligodendrocytes not only contain cytoplasmic gelsolin, but they also express a novel gelsolin isoform that we have named gelsolin-3. Cytoplasmic gelsolin, plasma gelsolin, and gelsolin-3 arise by alternative splicing from the same gene. The N-terminal amino acid sequence unique to gelsolin-3 is shown to be encoded by a single exon in a region previously thought to be an intron in the human gelsolin gene. In situ hybridization analysis confirmed that gelsolin-3 mRNA is localized primarily to oligodendrocytes in rat brain. In other tissues, gelsolin-3 shows a more restricted pattern of expression than cytoplasmic gelsolin. These data support the view that the gelsolin isoforms have differential roles in the regulation of the actin cytoskeleton.     

Interactions between the actin filament capping and severing protein gelsolin and the molecular chaperone CCT: evidence for nonclassical substrate interactions

CCT is a member of the chaperonin family of molecular chaperones and consists of eight distinct subunit species which occupy fixed positions within the chaperonin rings. The activity of CCT is closely linked to the integrity of the cytoskeleton as newly synthesized actin and tubulin monomers are dependent upon CCT to reach their native conformations. Furthermore, an additional role for CCT involving interactions with assembling/assembled microfilaments and microtubules is emerging. CCT is also known to interact with other proteins, only some of which will be genuine folding substrates. Here, we identify the actin filament remodeling protein gelsolin as a CCT-binding partner, and although it does not behave as a classical folding substrate, gelsolin binds to CCT with a degree of specificity. In cultured cells, the levels of CCT monomers affect levels of gelsolin, suggesting an additional link between CCT and the actin cytoskeleton that is mediated via the actin filament severing and capping protein gelsolin.     

Gelsolin, but not its cleavage, is required for TNF-induced ROS generation and apoptosis in MCF-7 cells

The tumor necrosis factor (TNF) can induce apoptosis in many cells including MCF-7 cells. To identify the genes responsible for TNF-induced apoptosis, we generated a series of TNF-resistant MCF-7 cell lines by employing retrovirus insertion-mediated random mutagenesis. In one of the resistant lines, gelsolin was found to be disrupted by viral insertion. Exogenous expression of gelsolin in this mutant cell line (Gel^mut) restored the sensitivity to TNF-induced cell death and knock-down of gelsolin by siRNA conferred MCF-7 cells with resistance to TNF, indicating that gelsolin is required for TNF-induced apoptosis. Interestingly, the resistance of Gel^mut cells to apoptosis induction is selective to TNF, since Gel^mut and wild-type cells showed similar sensitivity to other death stimuli that were tested. Furthermore, TNF-induced ROS production in Gel^mut cells was significantly decreased, demonstrating that gelsolin-mediated ROS generation plays a crucial role in TNF-induced apoptosis in MCF-7 cells. Importantly, caspase-mediated gelsolin cleavage is dispensable for TNF-triggered ROS production and subsequent apoptosis of MCF-7 cells. Our study thus provides genetic evidence linking gelsolin-mediated ROS production to TNF-induced cell death.     

Gelsolin蛋白在类风湿性关节炎和系统性红斑狼疮的临床诊断及疾病活动度评价中的意义

目的:分析gelsolin蛋白对类风湿性关节炎(rheumatoid arthritis,RA)和系统性红斑狼疮(systemic lupus erythematosus,SLE)的临床诊断及疾病活动度评价的意义。方法:采集RA 30名和SLE 47名及健康人群50名的临床资料及血清标本,定量Western Blot法检测血清gelsolin水平。分析gelsolin蛋白与RA和SLE患者临床表现及疾病活动度的相关性。结果:RA、SLE和正常对照组之间性别、年龄、血红蛋白、血小板、血红细胞、血白细胞之间没有显著差异;RA患者出现CRP、转氨酶、RF、CCP异常的阳性率明显高于SLE患者(P0.05);而SLE患者出现白蛋白、尿蛋白、尿红细胞、尿素氮、ANA、肌酐异常增高的几率高于RA患者(P0.05)。gelsolin蛋白在SLE和RA血清中的含量均显著低于正常人(P0.05),且RA患者含量更低(P0.05)。gelsolin蛋白滴度与RA的疾病活动度无明显相关性(r=0.089,P=0.652),而与SLE的疾病活动度呈显著负相关(r=0.646,P0.05)。gelsolin蛋白正常组RA患者的转氨酶升高、CRP、RF、CCP阳性率均显著高于SLE患者(P0.05)。gelsolin蛋白降低组SLE患者的白蛋白、尿蛋白、尿红细胞、尿素氮、ANA、肌酐阳性率显著高于RA患者(P0.05)。结论:gelsolin蛋白滴度检测可作为RA和SLE临床辅助诊断手段,其滴度变化可作为SLE疾病活动度进展的预判指标。     

Muscle gelsolin: isolation from heart tissue and characterization as an integral myofibrillar protein

A 92-kDa polypeptide present in rabbit and dog cardiac muscle was purified to homogeneity and some of its properties were investigated using biochemical and cytochemical approaches. The protein was found to be similar, if not identical to macrophage gelsolin; it cross-reacts immunologically with anti-rabbit macrophage gelsolin antibody, has a Ca2+-sensitive shortening effect on the actin filaments as judged by the high shear viscometry and sedimentation experiments, and has a similar amino acid composition. In addition, immunoblot and SDS polyacrylamide gel analysis of cardiac muscle extracts obtained at high and low ionic strength showed that this protein is tightly bound to myofibrils, both in the absence and presence of Ca2+, in ventricular as well as in atrial muscle cells. Indirect immunofluorescence microscopy revealed a striated gelsolin staining pattern analogous to that previously observed for the skeletal muscle gelsolin, suggesting that in the muscle cell this protein is sharing the same localisation as actin. Because of its severing and nucleating properties the gelsolin may play a major role in the organization, assembly and turnover of the thin filaments within the muscle cells.