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体外血小板生成。细胞骨架在巨核细胞破碎中的作用。

Blood platelet formation in vitro. The role of the cytoskeleton in megakaryocyte fragmentation.

作者信息

Tablin F, Castro M, Leven R M

机构信息

Department of Anatomy, School of Veterinary Medicine, University of California, Davis 95616.

出版信息

J Cell Sci. 1990 Sep;97 ( Pt 1):59-70. doi: 10.1242/jcs.97.1.59.

Abstract

We have developed a unique in vitro model that promotes differentiation of megakaryocytes into platelets. When megakaryocytes isolated from guinea pig bone marrow were cultured on hydrated rat tail collagen gels, cells spontaneously formed elongated, beaded processes that fragmented to yield cytoplasmic pieces with the same size and internal composition as individual platelets. Addition of nocodazole at the initiation of cultures blocked process formation, while addition of nocodazole to cells with previously established processes resulted in their retraction. The addition of taxol to cultures resulted in abnormally thick processes that were tightly adherent to the underlying substratum, and did not bead or fragment. Cytochalasin D accelerated process formation and fragmentation of megakaryocytes cultured on collagen gels by twofold. On the basis of these results, we propose a model for platelet formation in culture that involves the following steps: adherence of megakaryocytes to the underlying extracellular matrix; dilation of the demarcation membrane system and breakdown of the actin-rich peripheral zone; microtubule-based extension of pseudopodia, which are no longer adherent to the substratum; and fragmentation into platelets by the coalescence and fusion of demarcation membrane vesicles with the plasma membrane. We feel that this distinctive culture system closely approximates thrombocytopoiesis in vivo, thus allowing detailed elucidation of this important process.

摘要

我们开发了一种独特的体外模型,可促进巨核细胞向血小板分化。当从豚鼠骨髓中分离出的巨核细胞在水合大鼠尾胶原凝胶上培养时,细胞会自发形成细长的、串珠状的突起,这些突起会断裂,产生与单个血小板大小和内部组成相同的细胞质片段。在培养开始时添加诺考达唑会阻止突起的形成,而向已经形成突起的细胞中添加诺考达唑会导致突起缩回。向培养物中添加紫杉醇会导致异常粗大的突起紧密附着在下面的基质上,且不会形成串珠状或断裂。细胞松弛素D使在胶原凝胶上培养的巨核细胞的突起形成和断裂速度加快了两倍。基于这些结果,我们提出了一个培养中血小板形成的模型,该模型涉及以下步骤:巨核细胞附着于下面的细胞外基质;分界膜系统扩张,富含肌动蛋白的外周区分解;基于微管的伪足延伸,伪足不再附着于基质;分界膜囊泡与质膜合并和融合,分裂成血小板。我们认为这种独特的培养系统与体内血小板生成非常相似,从而能够详细阐明这一重要过程。

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