Alexafluor 488 phalloidin检测到的肌动蛋白纤维模式表明,在再生和非再生的啮齿动物脚趾中,细胞迁移相似。

Daniel A Neufeld, Steve Hosman, Tammy Yescas, Khalid Mohammad, Frances Day, Suleman Said
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引用次数: 0

摘要

虽然哺乳动物不能再生大多数附属物,但如果通过甲床进行截肢,它们能够再生脚尖。不同水平截肢后不同结果的原因尚不清楚。再生和非再生部位的细胞可能来自根本不同的组织。如果是这样,就可以发现不同的迁徙途径。为了鉴定可能的迁移细胞,在截肢后连续几天对大鼠和小鼠的再生和非再生脚趾进行显微镜载玻片。荧光标记的phalloidin结合聚合的f-肌动蛋白,用于识别肌动蛋白细丝和纤维。含有明显肌动蛋白束的细胞与含有弥漫性原纤维的细胞和没有可见纤维的细胞是可区分的。在截肢后再生和非再生指骨中,生殖器外环素标记相似。早在截肢后2天,在近端或远端水平上,伤口附近的许多皮下细胞都被phalloidin标记。含有应力纤维样束的标记皮下细胞的数量和强度随着时间的推移而迅速增加,并且在连续的时间内,细胞逐渐向远端延伸。大约7天,它们占据了再生和非再生指骨远端的伤口部位。大多数真皮细胞未标记,内皮细胞和骨髓细胞仅含有纤维肌动蛋白。Phalloidin标记不支持从再生和非再生截肢部位的不同组织迁移的概念。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Actin fiber patterns detected by Alexafluor 488 phalloidin suggest similar cell migration in regenerating and nonregenerating rodent toes.

Although mammals do not regenerate most appendages, they are able to regenerate toetips if the amputation occurs through the nail bed. The reasons for different outcomes following amputation at different levels are not understood. It is possible that cells at regenerating and nonregenerating sites migrate from fundamentally different tissues. If so, different migratory pathways could be detected. To identify putative migrating cells, microscope slides were made from both regenerating and nonregenerating toes of rats and mice on successive days after amputation. Fluorescent-labeled phalloidin, which binds polymerized f-actin, was used to identify actin filaments and fibers. Cells containing prominent actin bundles were distinguishable from those containing diffuse fibrils and those in which visible fibers were absent. Phalloidin labeling was similar in regenerating and nonregenerating digits after amputation. As early as 2 days after amputation at either proximal or distal levels, many cells of the hypodermis adjacent to the wound became labeled with phalloidin. The number and intensity of labeled hypodermal cells containing stress fiber-like bundles increased rapidly with time, and at successive times cells were seen progressively further distally. By approximately 7 days, they occupied the wound site immediately distal to bone of both regenerating and nonregenerating digits. Most dermal cells were unlabeled and endosteal and marrow cells contained only fibrillar actin. Phalloidin labeling does not support the concept of migration from different tissues in regenerating and nonregenerating amputation sites.

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