Shuster C B, Herman I M
Program in Cell, Molecular, and Developmental Biology, Tufts University Health Science Schools, Boston, Massachusetts 02111.
J Cell Biol. 1995 Mar;128(5):837-48. doi: 10.1083/jcb.128.5.837.
Whereas it has been demonstrated that muscle and nonmuscle isoactins are segregated into distinct cytoplasmic domains, the mechanism regulating subcellular sorting is unknown (Herman, 1993a). To reveal whether isoform-specific actin-binding proteins function to coordinate these events, cell extracts derived from motile (Em) versus stationary (Es) cytoplasm were selectively and sequentially fractionated over filamentous isoactin affinity columns prior to elution with a KCl step gradient. A polypeptide of interest, which binds specifically to beta-actin filament columns, but not to muscle actin columns has been conclusively identified as the ERM family member, ezrin. We studied ezrin-beta interactions in vitro by passing extracts (Em) over isoactin affinity matrices in the presence of Ca(2+)-containing versus Ca(2+)-free buffers, with or without cytochalasin D. Ezrin binds and can be released from beta-actin Sepharose-4B in the presence of Mg2+/EGTA and 100 mM NaCl (at 4 degrees C and room temperature), but not when affinity fractionation of Em is carried out in the presence of 0.2 mM CaCl2 or 2 microM cytochalasin D. N-acetyl-(leucyl)2-norleucinal and E64, two specific inhibitors of the calcium-activated protease, calpain I, protect ezrin binding to beta actin in the presence of calcium. Moreover, biochemical analysis of endothelial lysates reveals that a calpain I cleavage product of ezrin emerges when cell locomotion is stimulated in response to monolayer injury. Immunofluorescence analysis of leading lamellae reveals that anti-ezrin and anti-beta-actin IgGs can be simultaneously co-localized, extending the results of isoactin affinity fractionation of Em-derived extracts and suggesting that ezrin and beta-actin interact in vivo. To test the hypothesis that ezrin binds directly to beta-actin, we performed three sets of studies under a wide range of physiological conditions (pH 7.0-8.5) using purified pericyte ezrin and either alpha- or beta-actin. These included co-sedimentation, isoactin affinity fractionation, and co-immunoprecipitation. Results of these experiments reveal that purified ezrin does not directly bind to beta-actin filaments, either in solution or while isoactins are covalently cross-linked to Sepharose-4B. This is in contrast to our finding that ezrin and beta-actin could be co-immunoprecipitated or co-sedimented from Em-derived cell lysates. To explore whether calcium transients occur in cellular domains enriched in ezrin and beta-actin, we mapped cellular free calcium in endothelial monolayers crawling in response to injury.(ABSTRACT TRUNCATED AT 400 WORDS)
虽然已经证明肌肉和非肌肉同工肌动蛋白被分隔到不同的细胞质区域,但调节亚细胞分选的机制尚不清楚(赫尔曼,1993a)。为了揭示同工型特异性肌动蛋白结合蛋白是否发挥作用来协调这些事件,在通过KCl阶梯梯度洗脱之前,将源自运动(Em)与静止(Es)细胞质的细胞提取物在丝状同工肌动蛋白亲和柱上进行选择性和顺序分级分离。一种特别感兴趣的多肽,它特异性结合β-肌动蛋白丝柱,但不结合肌肉肌动蛋白柱,已被明确鉴定为ERM家族成员埃兹蛋白。我们通过在含Ca(2+)与不含Ca(2+)的缓冲液中,有或没有细胞松弛素D的情况下,将提取物(Em)通过同工肌动蛋白亲和基质来体外研究埃兹蛋白与β-肌动蛋白的相互作用。在Mg2+/EGTA和100 mM NaCl存在下(在4℃和室温),埃兹蛋白结合并可从β-肌动蛋白琼脂糖-4B上释放,但在0.2 mM CaCl2或2 microM细胞松弛素D存在下进行Em的亲和分级分离时则不能。钙激活蛋白酶钙蛋白酶I的两种特异性抑制剂N-乙酰-(亮氨酰)2-正亮氨酸和E64在钙存在下保护埃兹蛋白与β-肌动蛋白的结合。此外,对内皮裂解物的生化分析表明,当细胞运动因单层损伤而被刺激时,埃兹蛋白的钙蛋白酶I裂解产物会出现。对前沿薄片的免疫荧光分析表明,抗埃兹蛋白和抗β-肌动蛋白IgG可以同时共定位,扩展了源自Em的提取物的同工肌动蛋白亲和分级分离结果,并表明埃兹蛋白和β-肌动蛋白在体内相互作用。为了检验埃兹蛋白直接结合β-肌动蛋白的假设,我们在广泛的生理条件(pH 7.0 - 8.5)下使用纯化的周细胞埃兹蛋白和α-或β-肌动蛋白进行了三组研究。这些研究包括共沉降、同工肌动蛋白亲和分级分离和共免疫沉淀。这些实验结果表明,纯化的埃兹蛋白无论是在溶液中还是在同工肌动蛋白与琼脂糖-4B共价交联时,都不直接结合β-肌动蛋白丝。这与我们发现埃兹蛋白和β-肌动蛋白可以从源自Em的细胞裂解物中共免疫沉淀或共沉降形成对比。为了探索在富含埃兹蛋白和β-肌动蛋白的细胞区域是否发生钙瞬变,我们绘制了响应损伤而爬行的内皮单层中的细胞游离钙分布图。(摘要截短至400字)
