Cytoplasmic dynein colocalizes with melanosomes in normal human melanocytes

动力蛋白 黑素体 微管 细胞生物学 细胞质 生物 动态素 运动蛋白 细胞骨架 免疫荧光 分子马达 微管相关蛋白 肌动蛋白 细胞 黑色素 生物化学 遗传学 抗体
作者
Garnet Vancoillie,Jo Lambert,Aat A. Mulder,Henk K. Koerten,A. Mieke Mommaas,Patric Van Oostveldt,Jean Naeyaert
出处
期刊:British Journal of Dermatology [Oxford University Press]
卷期号:143 (2): 298-306 被引量:42
标识
DOI:10.1046/j.1365-2133.2000.03654.x
摘要

Background Melanocytic dendrites consist of a central core of microtubules and a subcortical actin network. Several studies provide arguments supporting the hypothesis that actin‐based and microtubule‐based motor proteins co‐operate in melanosome transport towards the dendrite tips. Melanosomes can move bidirectionally along microtubules in vitro, and in murine melanocytes, they move towards the cell periphery and back again. Microtubules have a fast‐growing plus end and a slow‐growing minus end . Microtubule‐associated motor proteins move unidirectionally either towards the plus or towards the minus end. However, it is not known which motor protein is responsible for minus end‐directed movement of melanosomes. Objectives We aimed to investigate the in vitro expression of the minus end‐directed motor protein cytoplasmic dynein in normal human epidermal melanocytes, keratinocytes and dermal fibroblasts. Methods Reverse transcription–polymerase chain reaction and Northern blot analysis were used. In addition, an attempt to obtain insight into the subcellular localization of cytoplasmic dynein, immunofluorescence studies and immunogold electron microscopic studies were performed. Results The three different forms of cytoplasmic dynein heavy chain were expressed in all studied skin cells. Immunofluorescence staining showed similar punctate distributions for dynein heavy chain 1 and dynein heavy chain 2 in melanocytes, with accentuation in the perinuclear area and dendrite tips. Double labelling with a melanosome marker showed apparent co‐localization of both dynein heavy chains 1 and 2 with melanosomes in the perinuclear area and dendrite tips. For the dynein intermediate chain of 74 kDa, again a punctate staining pattern was seen with intense centrosomal staining. A close association of dynein intermediate chain 74 and α‐tubulin with the melanosome surface was detected using immunogold electron microscopy. Conclusions The colocalization of different subunits of the cytoplasmic dynein complex with melanosomes is consistent with the hypothesis that this motor protein supports minus end‐directed melanosome movement along microtubules.

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