Parsey M V, Lewis G K
Department of Microbiology and Immunology, University of Maryland Medical School, Baltimore 21201.
J Immunol. 1993 Aug 15;151(4):1881-93.
T cell activation via CD3/Ti linked pathways results in the polymerization and reorganization of actin. However, little is known about the morphology and temporal appearance of filamentous actin (F-actin) after activation. Similarly, little is known about the relationship between F-actin and changes in cell shape or other parameters of activation, such as the appearance of proteins newly phosphorylated on tyrosine, that occur after stimulation via the CD3/Ti complex. Accordingly, we have characterized changes in cell shape and F-actin morphology occurring in the Jurkat T cell leukemia attached to the surface of culture vessels by immobilized anti-CD3 antibodies (OKT3, UCHT-1, SPV-T3b). These antibodies induced activation within 30 min as measured by increased protein tyrosine kinase activity and conversion of the proto-oncogene product, lck, from 56 kDa to 60 kDa (p56lck conversion), and after 12 to 96 h as measured by growth arrest and, in some experiments, IL-2 production. Activation was not seen when cells were attached to the substrates using antibodies directed to other cell surface proteins including CD71 (transferrin receptor), CD7, and CD11a (LFA-1), demonstrating the specificity of activation for immobilized anti-CD3 antibodies. Temporal changes in cell shape and F-actin morphology were characterized in Jurkat cells attached by immobilized anti-CD3 antibodies (stimulatory antibodies) and compared with the patterns obtained obtained in Jurkat cells attached by antibodies specific for the other markers (nonstimulatory antibodies). In these experiments, Jurkat cells were incubated with antibody-coated substrates for 1 to 30 min at 37 degrees C and actin rearrangements were visualized on fixed, detergent-permeabilized cells using rhodamine-conjugated phalloidin. Analysis of cell shape and F-actin morphology during the first 30 min of activation revealed a unique pattern that was observed only when cells were stimulated with anti-CD3 antibodies. Jurkat cells attached by either stimulatory or nonstimulatory antibodies reorganized their actin similarly after the first minute of culture, as characterized by the formation of small, F-actin rich pseudopods at the sites of attachment. After 5 min of culture in cells attached by stimulatory antibodies, the actin was polymerized into a dense collar rimming the inner edge of the cell. From 15 to 60 min, this collar was replaced by numerous F-actin rich, branched pseudopods. These branched pseudopods were larger and had longer microfilament bundles than their earlier counterparts. By contrast, in cells attached by nonstimulatory antibodies, the initial configuration was maintained for at least 60 min, except that a decrease in microfilament bundle length was noted.(ABSTRACT TRUNCATED AT 400 WORDS)
通过CD3/Ti连接途径激活T细胞会导致肌动蛋白的聚合和重排。然而,关于激活后丝状肌动蛋白(F-肌动蛋白)的形态和出现时间知之甚少。同样,关于F-肌动蛋白与细胞形状变化或其他激活参数之间的关系也知之甚少,例如通过CD3/Ti复合物刺激后出现的酪氨酸新磷酸化蛋白。因此,我们已经描述了通过固定化抗CD3抗体(OKT3、UCHT-1、SPV-T3b)附着在培养容器表面的Jurkat T细胞白血病细胞中细胞形状和F-肌动蛋白形态的变化。这些抗体在30分钟内诱导激活,这通过蛋白质酪氨酸激酶活性增加以及原癌基因产物lck从56 kDa转化为60 kDa(p56lck转化)来衡量,并且在12至96小时后通过生长停滞来衡量,在一些实验中还通过白细胞介素-2的产生来衡量。当细胞使用针对其他细胞表面蛋白(包括CD71(转铁蛋白受体)、CD7和CD11a(淋巴细胞功能相关抗原-1))的抗体附着在底物上时,未观察到激活,这证明了固定化抗CD3抗体激活的特异性。通过固定化抗CD3抗体(刺激抗体)附着的Jurkat细胞中细胞形状和F-肌动蛋白形态的时间变化进行了表征,并与通过针对其他标志物的抗体(非刺激抗体)附着的Jurkat细胞中获得的模式进行了比较。在这些实验中,将Jurkat细胞与抗体包被的底物在37℃下孵育1至30分钟,并使用罗丹明偶联的鬼笔环肽在固定的、经去污剂通透处理的细胞上观察肌动蛋白重排。对激活的前30分钟内细胞形状和F-肌动蛋白形态的分析揭示了一种独特的模式,该模式仅在细胞用抗CD3抗体刺激时观察到。在培养的第一分钟后,通过刺激或非刺激抗体附着的Jurkat细胞以类似的方式重组其肌动蛋白,其特征是在附着部位形成小的、富含F-肌动蛋白的伪足。在用刺激抗体附着的细胞中培养5分钟后,肌动蛋白聚合成围绕细胞内边缘的致密环。从15到60分钟,这个环被许多富含F-肌动蛋白的分支伪足所取代。这些分支伪足比早期的伪足更大,微丝束更长。相比之下,在用非刺激抗体附着的细胞中,初始构型至少维持60分钟,只是微丝束长度有所减少。(摘要截短至400字)
