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溶酶体在通透巨噬细胞中沿微管的径向运动。

Radial movement of lysosomes along microtubules in permeabilized macrophages.

作者信息

Swanson J A, Locke A, Ansel P, Hollenbeck P J

机构信息

Department of Anatomy and Cellular Biology, Harvard Medical School, Boston, MA 02115.

出版信息

J Cell Sci. 1992 Sep;103 ( Pt 1):201-9. doi: 10.1242/jcs.103.1.201.

DOI:10.1242/jcs.103.1.201
PMID:1429905
Abstract

In murine bone marrow-derived macrophages, lysosomes often form tubulovesicular compartments, whose extended distribution in the cytoplasm depends on the integrity of cytoplasmic microtubules. When macrophages with fluorescently labeled lysosomes were plated onto coverslips opsonized with IgG, they engaged that surface in a phagocytic response (frustrated phagocytosis). The tubular lysosomal compartment of these cells collected in a central, perinuclear region, despite the continued presence of a radiating array of cytoplasmic microtubules. Using methods developed in the study of melanophores, we permeabilized macrophages engaged in frustrated phagocytosis, then re-activated lysosome extension along microtubules. Permeabilization was selective for plasma membranes, in that high molecular weight probes such as trypan blue or IgG could enter cells, while fluorescent probes previously loaded into lysosomes via endocytosis remained contained therein. Addition of 2 mM ATP, GTP or UTP to these permeabilized cell models produced centrifugal extension of tubular lysosomes. Selective depletion of ATP, using Escherichia coli glycerol kinase, inhibited ATP-dependent extension but not that which occurred with GTP or UTP, indicating that the mechanism of radial movement can use any of these three nucleotide triphosphates. Extension was independent of pH between 6.8 and 7.4, and was inhibited by AMP-PNP and by GMP-PNP. Depolymerization of cytoplasmic microtubules with nocodazole prevented subsequent ATP-inducible lysosome extension, whereas preincubation of cells with cytochalasin D did not inhibit the response. These results are consistent with the in vitro mechanochemical properties of kinesin (Cohn et al., 1989), and support earlier evidence, obtained in living cells, that kinesin is the mechanochemical motor of lysosome extension along microtubules in macrophages.

摘要

在小鼠骨髓来源的巨噬细胞中,溶酶体常常形成管状囊泡区室,其在细胞质中的广泛分布依赖于细胞质微管的完整性。当将带有荧光标记溶酶体的巨噬细胞接种到用免疫球蛋白G(IgG)调理过的盖玻片上时,它们会以吞噬反应(受挫吞噬作用)附着于该表面。尽管细胞质微管呈放射状排列持续存在,但这些细胞的管状溶酶体区室会聚集在细胞核周围的中央区域。利用在黑素细胞研究中开发的方法,我们使参与受挫吞噬作用的巨噬细胞透化,然后重新激活溶酶体沿微管的延伸。透化对质膜具有选择性,因为诸如台盼蓝或IgG等高分子量探针可以进入细胞,而先前通过内吞作用加载到溶酶体中的荧光探针仍保留在其中。向这些透化的细胞模型中添加2 mM三磷酸腺苷(ATP)、三磷酸鸟苷(GTP)或三磷酸尿苷(UTP)会使管状溶酶体产生离心延伸。使用大肠杆菌甘油激酶选择性耗尽ATP,可抑制依赖ATP的延伸,但不影响由GTP或UTP引发的延伸,这表明径向运动机制可以使用这三种三磷酸核苷酸中的任何一种。延伸在pH值6.8至7.4之间与pH无关,并受到腺苷-5'-三磷酸-γ-亚胺(AMP-PNP)和鸟苷-5'-三磷酸-γ-亚胺(GMP-PNP)的抑制。用诺考达唑使细胞质微管解聚可阻止随后ATP诱导的溶酶体延伸,而用细胞松弛素D对细胞进行预孵育并不抑制该反应。这些结果与驱动蛋白的体外机械化学特性一致(科恩等人,1989年),并支持在活细胞中获得的早期证据,即驱动蛋白是巨噬细胞中溶酶体沿微管延伸的机械化学动力蛋白。

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Radial movement of lysosomes along microtubules in permeabilized macrophages.溶酶体在通透巨噬细胞中沿微管的径向运动。
J Cell Sci. 1992 Sep;103 ( Pt 1):201-9. doi: 10.1242/jcs.103.1.201.
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