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外源性层粘连蛋白对腹水型肝癌细胞内微丝组装和细胞游动的作用 总被引:3,自引:1,他引:2
本文研究外源性层粘连蛋白与癌细胞膜上受体结合调节胞内肌动蛋白微丝组装与改变细胞游动之间的关系,以及影响膜上层粘连蛋白受体的侧向扩散运动及膜脂分子流动性变化之间的关系.用各种荧光技术,如荧光显微米,荧光漂白恢复技术和荧光流式细胞术得到了明显的证据.层粘连蛋白与肝癌细胞膜有结合,使分散的腹水肝癌细胞粘连聚集,并膜下周动蛋白微丝增加,当把癌细胞分开则细胞从原位游动很大距离.如不分离粘连的细胞可减少其脱落和转移.层粘连蛋白与受体结合则受体的侧向扩散系数减小,膜脂流动性降低,使膜上分子运动受影响,对癌的生长不利. 相似文献
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配体蛋白与细胞膜受体蛋白结合后,可引起膜受体的构象与膜脂的有序性变化.本文研究外源性层粘连蛋白与腹水肝癌细胞膜受体结合后膜热量变化,膜序参数改变和膜电荷及细胞迁移率的变更.就膜蛋白构象与膜脂有序性以及膜电荷等方面改变的生理意义与层粘连蛋白抗癌细胞脱落转移寻找理论关系.本文应用微量量热法、顺磁共振和细胞电泳等技术,得知层粘连蛋白与癌细胞膜作用后细胞膜有放热效应,膜流动性增大,细胞电泳动变慢.癌细胞膜的这些变化对于限制癌的恶性生长与脱落均起重要作用. 相似文献
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荧光标记法检测不同毒物对细胞骨架的影响 总被引:2,自引:0,他引:2
细胞骨架(Cytoskeleton)主要由微管(Microtubule,MT)、微丝(Microfilament,MF)以及中间丝(Intermediate filament,IF)这三种类型组成。它们在细胞的形态维持、物质运输、信号转导、能量转换及细胞的运动和分裂等多个过程中发挥着重要的作用。其中,由肌动蛋白组成的微丝是真核细胞中含量最丰富的一种蛋白复合体,以解聚时的球状肌动蛋白G-actin(Globular actin)或聚合时的纤丝状肌动蛋白F-actin(Filamen-tous actin)形式存在。正常细胞中肌动蛋白两种形态的转换处于动态平衡,共同行使细胞的变形运动、胞质分裂、基质附着和胞间连接等多… 相似文献
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微丝骨架在细胞的生命活动中具有重要的功能,而其动态的解聚聚合特性是其实现功能的前提. 丝束蛋白(fimbrin/plastin)做为微丝结合蛋白质,是微丝骨架的重要调控因子之一,含有2个肌动蛋白结合结构域,目前对其结合微丝的机制并不清楚. 本文以烟草丝束蛋白的肌动蛋白结合结构域2(NtFAbd2) 为研究对象,通过原核细胞表达纯化NtFAbd2,利用体外沉淀法分析发现,NtFAbd2能够与微丝结合;利用激光共聚焦扫描显微镜分析发现,在烟草BY-2悬浮细胞内,NtAbd2-GFP与微丝共分布,这些结果为深入分析植物丝束蛋白的作用机制提供了新的数据. 相似文献
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肌动蛋白相关蛋白2/3复合体的结构、功能与调节 总被引:3,自引:0,他引:3
微丝参与了细胞形态维持及细胞运动等多种重要的细胞过程。微丝由肌动蛋白单体组装而成 ,肌动蛋白相关蛋白 2 / 3(Arp2 /Arp3,Arp2 / 3)复合体在微丝形成过程中起重要作用。Arp2 / 3复合体由 7个亚单位组成 ,在细胞内受到多种核化促进因子的调节 ,并与这些因子协同作用来调节肌动蛋白的核化。Arp2 / 3复合体结构、功能及调节的研究对于阐明微丝形成机制及细胞骨架与某些信号分子的关系有重要意义。 相似文献
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皮动蛋白及微丝相关蛋白2/3复合物介导的细胞运动的分子机制 总被引:2,自引:0,他引:2
皮动蛋白(cortactin)是一种含有特殊重复序列结构域的微丝肌动蛋白结合蛋白,它直接参与了细胞皮层(cortex)微丝细胞骨架的组建。它又是细胞内Src类酪氨酸蛋白激酶的主要底物之一,代表了一类高度保守的胞内皮层信号蛋白质家族。近几年来,对于细胞运动分子机制的研究取得很大进展,利用组织培养细胞进行的体外实验证明。皮动蛋白能够活化微丝相关蛋白2/3复合物(actin related protein 2/3 complex,Arp2/3 complex),调控皮层微丝细胞骨架的组装,在细胞运动过程中具有重要作用。 相似文献
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细胞骨架由微丝、微管及中等纤维组成受不同蛋白因子调控以不同方式组装成不同直径的纤维 ,遍布于一切细胞 ,决定细胞的形状 ,赋予其抗压强度 ,对细胞器及大分子进行空间组织 ,实现胞内的能量转换。在肌动蛋白 (actin)组装成张力纤维和张力纤维解离成肌动蛋白单体过程中有多种蛋白因子参与调控 ,从而使细胞骨架处于一个生理的动态平衡中 ,执行和完成不同的生化反应。在众多的调控蛋白中 ,肌动蛋白集束调控蛋白因子 (actinbundlingprotein)不仅参与肌动蛋白结构调节 ,还与细胞内信号传导有密切关系。已发现的肌动蛋… 相似文献
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染色质的组成成分,组蛋白和非组蛋白在特异的蛋白激酶作用下可以发生磷酸化修饰,组蛋白和非组蛋白的磷酸化和脱磷酸化可能在染色质的结构,基因表达以及DNA复制中起着重要的作用。本文比较是小鼠腹水型肝癌细胞核和正常小鼠肝细胞核内酸溶性蛋白质及其磷酸化的差异。正常小鼠肝细胞核酸溶性蛋白质的电泳染色图谱有一条明显可见的组蛋白H_1~0蛋白带,而对小鼠腹水型肝癌来说,此带极浅,但在腹水型肝癌细胞核酸溶性蛋白质的电泳染色图谱上可见到表观分子量约为68K的一条蛋白带,而正常小鼠肝未见此带。此外,从电泳胶片~(32)P放射自显影图谱可见腹水型肝癌组蛋白H_1,H_2A和非组蛋白带Ⅱ(MW43K),带Ⅲ(MW.67K)带Ⅳ(M.w.97K)磷酸化程度明显高于正常小鼠肝。 相似文献
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Tiuriaeva II Mirgorodskaia OA Cherepanova OA Podol'skaia EP Novikov AV Khodorkovskiĭ MA Ivanov VA 《Tsitologiia》2005,47(2):150-162
Cell dysdifferentiation during neoplastic transformation is a crucial problem of cell biology and oncology. Antigenic diversion of cancer cells is a typical characteristic of dysdifferentiation. It involves the appearance of antigens which are unusual for normal tissue of this type. Components organospecific for membrane proteins of normal kidney were previously found among plasma membrane proteins of hepatocellular rat tumors, rat hepatocytes after carcinogen treatment, and regenerating liver, respectively. In the present work we showed that a protein with mol. weight about 200 kDa reacting with laminin-1 immunoserum is the basic component of plasma membranes of the rat Zajdela hepatoma cells, which is responsive for organospecific anti-kidney immunoserum in Western blot. A mass-spectrometer analysis of trypsin proteolysis fragments was carried out in SDS-PAGE slices containing the investigated component. The analysis showed the presence of beta1, beta2 and alpha4 laminin chains peptides. The component with mol. weight about 180 kDa, found in the Western blot with laminin-1 immunoserum, was also subjected to the mass spectrometer analysis. As a result, a gamma1 laminin chain was found. An increased amount of laminin was revealed in the ascitic liquid and sera of rat with developed Zajdela hepatoma, in comparison with sera of normal rats. In addition, we found the appearance of laminin on the hepatocyte surface on the 4th day after hepatocarcinogen injection (N-diethylnitrosamine, DENA). Thus, for the first time tumor associated antigens were revealed and identified in the structure of plasma membranes of Zajdela hepatoma cells, being specific to rat kidneys. Our results allow to conclude that in the process of carcinogenesis in rat liver laminin synthesis occurs, which is also characteristic of the rat hepatoma Zajdela cells. 相似文献
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K A Lebedev D R Kaulen V V Khorobrykh G N D'iakov A V Simonova 《Biulleten' eksperimental'no? biologii i meditsiny》1977,84(12):712-714
The action of antitumour sera on the adhesive properties of the L-cells and the cells of Ehrlich's ascitic carcinoma. It was shown that after the treatment with immune sera the tumour cells lost their capacity to form rosettes with sheep red blood cells, to adhere to plastics and glass; when administered into the mouse organism these cells were worse retained in the lungs, spleen and the liver. The data obtained indicated that the antibodies could play a significant role in the tumour cell metastasis. 相似文献
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鼠肝细胞癌变中DNA甲基化作用的研究 总被引:4,自引:0,他引:4
Activity of DNA methylase and DNA methylation level were measured from normal mouse liver, mouse liver charged with H22a ascitic hepatoma and H22a ascitic hepatoma cell by measuring incorporation of H3-methyl. S-Adenosyl-3H-methyl-methionine (3H-SAM) was used as methyl donor. DNA methylation level of different cells were measured by HP-LC. DNA methylase activity and DNA methylation level of H22a ascitic hepatoma, mouse liver charged with H22a ascitic hepatoma are lower than normal mouse liver. Treatments of antitumor drugs lead to a rising of DNA methylase activity of tumor cell, however, the DNA methylation level of tumor cell has not rised after such treatments. 相似文献
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To explore potential molecular chaperones involved in the intracellular assembly of laminin chains, bovine aortic endothelial
cells were treated with a thiol cleavable divalent cross-linking reagent, dithio-bis-(succinimidylpropionate), and cellular
proteins cross-linked to laminin chains were co-immunoprecipitated with anti-laminin antiserum. Sodium dodecylsulfate (SDS)
gel electrophoresis of the precipitate under reducing condition showed polypeptides with estimated sizes of 80, 60 and 50
kDa together with laminin chains. Two dimensional electrophoresis, in which non-reducing and reducing SDS electrophoresis
were combined, suggested that many molecules of these polypeptides were cross-linked to each laminin chain. Sepharose CL-4B
beads conjugated with E8 fragment of mouse laminin-1 was prepared. Affinity chromatography with the beads of microsomal proteins
from rat liver showed that Bip and HSP70 associated to laminin chains and dissociated upon ATP hydrolysis. Protein-disulfide
isomerase also showed affinity to the column. GRP94 and calnexin showed strong affinity and were washed out only with a detergent
solution. Thus, many molecular chaperones are suggested to be involved in the intracellular assembly of laminin chains.
This revised version was published online in June 2006 with corrections to the Cover Date. 相似文献
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Directed cell migration requires continuous cycles of protrusion of the leading edge and contraction to pull up the cell rear. How these spatially distributed processes are coordinated to maintain a state of persistent protrusion remains unknown. During wound healing responses of epithelial sheets, cells along the wound edge display two distinct morphologies: ‘leader cells’ exhibit persistent edge protrusions, while the greater majority of ‘follower cells’ randomly cycle between protrusion and retraction. Here, we exploit the heterogeneity in cell morphodynamic behaviors to deduce the requirements in terms of cytoskeleton dynamics for persistent and sporadic protrusion events. We used quantitative Fluorescent Speckle Microscopy (qFSM) to compare rates of F-actin assembly and flow relative to the local protrusion and retraction dynamics of the leading edge. Persistently protruding cells are characterized by contractile actomyosin structures that align with the direction of migration, with converging F-actin flows interpenetrating over a wide band in the lamella. Conversely, non-persistent protruders have their actomyosin structures aligned perpendicular to the axis of migration, and are characterized by prominent F-actin retrograde flows that end into transverse arcs. Analysis of F-actin kinetics in the lamellipodia showed that leader cells have three-fold higher assembly rates when compared to followers. To further investigate a putative relationship between actomyosin contraction and F-actin assembly, myosin II was inhibited by blebbistatin. Treated cells at the wound edge adopted a homogeneously persistent protrusion behavior, with rates matching those of leader cells. Surprisingly, we found that disintegration of actomyosin structures led to a significant decrease in F-actin assembly. Our data suggests that persistent protrusion in these cells is achieved by a reduction in overall F-actin retrograde flow, with lower assembly rates now sufficient to propel forward the leading edge. Based on our data we propose that differences in the protrusion persistence of leaders and followers originate in the distinct actomyosin contraction modules that differentially regulate leading edge protrusion-promoting F-actin assembly, and retraction-promoting retrograde flow. 相似文献
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The circadian clock in the brain coordinates the phase of peripheral oscillators that regulate tissue-specific physiological outputs. Here we report that circadian variations in the expression and activity of Cu/Zn superoxide dismutase (SOD1; EC 1.15.1.1) are present in liver homogenates from mice. The SOD1 mRNA expression from wild-type (WT) mice peaked at Zeitgeber Time 9 (ZT9; 9 h after lights-on time). While there was no rhythmicity in that from period2 (per2) gene knockout (P2K) mice, the level of SOD1 from per1/per2 double knockout (DKO) mice was significantly elevated at ZT5. The enzyme activity of SOD1 was also rhythmic in the mouse liver. Moreover, the total amount of the SOD1 exhibited a rhythmic oscillation with a peak at ZT9 in the liver from WT mice. We also found that tert-butylhydroperoxide (t-BHP)-induced oxidative damage in both WT and P2K mouse embryonic fibroblast (MEF) cells resulted in the up-regulation of SOD1 levels. Our data suggest that the expression of an important antioxidant enzyme, SOD1, is under circadian clock control and that mice are more susceptible to oxidative stress depending on the time of day. 相似文献
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Most interstitia between epithelial and endothelial cells contain basal laminae (BLs), as defined by electron microscopy. However, in liver, the sinusoidal interstitium (called space of Disse) between hepatocytes and sinusoidal endothelial cells (SECs) lacks BLs. Because laminins are major components of BLs throughout the body, whether laminins exist in sinusoids has been a controversial issue. Despite recent advances, the distribution and expression of laminin chains have not been well defined in mammalian liver. Here, using a panel of antibodies, we examined laminins in normal and regenerating mouse livers. Of alpha chains, alpha5 was widely observed in all BLs except for sinusoids, while the other alpha chains were variously expressed in Glisson's sheath and central veins. Laminin gamma1 was also distributed to all BLs except for sinusoids. Although the beta2 chain was observed in all BLs and sinusoids, the expression of beta1 chain was restricted to Glisson's sheath. Detailed analysis of regenerating liver revealed that alpha1 and gamma1 chains appeared in sinusoids and were produced by stellate cells. The staining of alpha1 and gamma1 chains reached its maximum intensity at 6 days after two-thirds partial hepatectomy (PHx). Moreover, in vitro studies showed that alpha1-containing laminin promoted spreading of sinusoidal endothelial cells (SECs) isolated from normal liver, but not other hepatic cells. In addition, SECs isolated from regenerating liver elongated pseudopodia on alpha1-containing laminin more so than did cells from normal liver. The transient expression of laminin alpha1 may promote formation of sinusoids after PHx. 相似文献
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Analysis of the assembly of laminin and the laminin-entactin complex with laminin chain specific monoclonal and polyclonal antibodies 总被引:1,自引:0,他引:1
Antibodies specific for the A, B1, and B2 chains of laminin have been obtained and characterized. Lam V, a rat X mouse monoclonal antibody, was obtained by immunizing Lewis rats with the extracellular matrix derived from the mouse endodermal line M1536-B3. The antibody was shown to recognize a conformation-sensitive epitope present on the A chain of laminin. The antibody exhibited high avidity for native laminin and uncomplexed newly synthesized laminin A chains. cDNA clones in the vector lambda-gt11 containing sequences for the B1 and B2 chains of laminin were shown to synthesize beta-galactosidase fusion proteins in the host cells induced with IPTG. The fusion protein F3 contained amino acid residues 822-1765 of the B1 chain of mouse laminin, and the fusion protein E4 contained 219 amino acids at the carboxyl terminus of the B2 chain of rat laminin. These two fusion proteins were used to obtain rabbit polyclonal antibodies which were characterized for their specificity and ability to immunoprecipitate laminin and the B chains of laminin. The chain-specific antibodies were used to analyze the assembly and processing of laminin in the mouse endodermal cell line M1536-B3. The results indicated that the covalent assembly of the A and B chains of laminin was initiated as early as 3 min after labeling cells. At this time point uncomplexed A chain of laminin could be observed even though there was an excess of B1 and B2 chains. As early as 4 min after labeling monomeric, dimeric, and oligomeric forms of the B chains of laminin were observed.(ABSTRACT TRUNCATED AT 250 WORDS) 相似文献