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电穿孔对胶原蛋白基质中培养的角膜成纤维细胞微管蛋白细胞骨架及定向迁移的影响。

Effects of electroporation on the tubulin cytoskeleton and directed migration of corneal fibroblasts cultured within collagen matrices.

作者信息

Harkin D G, Hay E D

机构信息

Department of Cell Biology, Harvard Medical School, Boston, Massachusetts 02115-5729, USA.

出版信息

Cell Motil Cytoskeleton. 1996;35(4):345-57. doi: 10.1002/(SICI)1097-0169(1996)35:4<345::AID-CM6>3.0.CO;2-5.

DOI:10.1002/(SICI)1097-0169(1996)35:4<345::AID-CM6>3.0.CO;2-5
PMID:8956005
Abstract

Electroporation provides a useful method for loading fibroblasts with fluorescent probes for the cytoskeleton, but the possible deleterious effects of this loading technique on cell motility are unknown. We have used conventional and confocal microscopy of living cells and immunohistochemistry to examine the migration and cytoskeleton of chick embryo corneal fibroblasts electroporated while cultured within collagen gels. Fibroblasts cultured in collagen (1 mg/ml) are successfully electroloaded (0.5-1.0 kVcm-1/960 microF in DMEM/F12/20 mM Hepes, pH 7.2) with dextran (4-150 kDa) and immunoglobulin, but subsequently display uncoordinated pseudopodia and hence are unable to migrate effectively in any one direction. The lack of directed movement is due to depolymerization of microtubules and/or a perinuclear collapse of vimentin filaments, seemingly caused by millimolar levels of Ca2+ ions derived from culture medium following electroporation. Fibroblasts loaded in a buffer which resembles intracellular fluid (< or = 10 microM Ca2+) maintain their cytoskeleton and continue to migrate, when returned to culture medium within 10 min. Using this novel approach, we have loaded fibroblasts migrating through extracellular matrix (ECM) with rhodamine phalloidin and monitored the behavior of the labeled actin cortex by confocal microscopy. During migration phalloidin-actin accumulates near the base of pseudopodia and at the rear of the cell where it is subsequently left behind. We conclude that electroporation is a valuable technique for loading fibroblasts to study migration within ECM, provided that the conditions used support stability of the tubulin cytoskeleton.

摘要

电穿孔为用荧光探针加载成纤维细胞的细胞骨架提供了一种有用的方法,但这种加载技术对细胞运动可能产生的有害影响尚不清楚。我们使用活细胞的传统显微镜和共聚焦显微镜以及免疫组织化学方法,来检查在胶原凝胶中培养时经电穿孔处理的鸡胚角膜成纤维细胞的迁移和细胞骨架情况。在胶原(1毫克/毫升)中培养的成纤维细胞,在DMEM/F12/20毫摩尔HEPES(pH 7.2)中成功地用电穿孔法加载了葡聚糖(4 - 150千道尔顿)和免疫球蛋白(0.5 - 1.0千伏/厘米/960微法),但随后显示出伪足不协调,因此无法在任何一个方向上有效地迁移。缺乏定向运动是由于微管解聚和/或波形蛋白丝在核周塌陷,这似乎是由电穿孔后培养基中毫摩尔水平的钙离子引起的。在类似于细胞内液(≤10微摩尔钙)的缓冲液中加载的成纤维细胞,如果在10分钟内回到培养基中,就能维持其细胞骨架并继续迁移。使用这种新方法,我们用罗丹明鬼笔环肽加载了在细胞外基质(ECM)中迁移的成纤维细胞,并通过共聚焦显微镜监测标记的肌动蛋白皮层的行为。在迁移过程中,鬼笔环肽 - 肌动蛋白在伪足基部附近和细胞后部积累,随后留在那里。我们得出结论,电穿孔是一种用于加载成纤维细胞以研究其在ECM中迁移的有价值的技术,前提是所使用的条件支持微管蛋白细胞骨架的稳定性。

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