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小鼠耳器官培养中表皮细胞的增殖。

The proliferation of epidermal cells in mouse ear organ culture.

作者信息

Gradwohl P R

出版信息

Arch Dermatol Res. 1978 Dec 1;263(3):273-81. doi: 10.1007/BF00446944.

Abstract

Mouse ear fragments were cultured for up to 1 day in a chemically defined fluid medium and for 2-3 days in a solid Agar medium. Within 24 h of incubation, the epidermal cells were found to migrate towards the cut edges, a process which led to an epithelialization of the denuded surface. Concomitantly, the epidermal cell proliferation was enhanced: an entry of increasing numbers of interfollicular cells into S phase occurred after 7-10 h of incubation and was maximal around the 20th h. Correspondingly, the mitotic rate rose after 20 h. During an incubation period of 48-72 h in solid medium, the mitotic activity of the proliferating tissues in mouse ear skin continued, and the interfollicular epidermis in the proximity of the cut edges became hyperplastic. Thus, mouse ear epidermis kept in this organ culture seems to resemble a wounded epidermis in vivo. Epidermal cell proliferation was studied by determining (a) the mitotic rate and (b) the incorporation of tritiated thymidine by means of liquid scintillation spectrometry and autoradiography. Various factors affecting the incorporation of tritiated thymidine were investigated, and it was concluded that liquid scintillation spectrometry proves to be a rapid and suitable method for determining the effects of both growth-promoting and growth-inhibiting agents on epidermal cell proliferation.

摘要

将小鼠耳部组织块在化学成分明确的液体培养基中培养长达1天,然后在固体琼脂培养基中培养2 - 3天。在培养24小时内,发现表皮细胞向切口边缘迁移,这一过程导致裸露表面上皮化。与此同时,表皮细胞增殖增强:培养7 - 10小时后,越来越多的毛囊间细胞进入S期,在第20小时左右达到最大值。相应地,有丝分裂率在20小时后上升。在固体培养基中培养48 - 72小时期间,小鼠耳部皮肤增殖组织的有丝分裂活动持续,切口边缘附近的毛囊间表皮增生。因此,保存在这种器官培养中的小鼠耳部表皮似乎类似于体内受伤的表皮。通过(a)有丝分裂率和(b)借助液体闪烁光谱法和放射自显影法测定氚标记胸腺嘧啶核苷的掺入情况来研究表皮细胞增殖。研究了影响氚标记胸腺嘧啶核苷掺入的各种因素,得出结论:液体闪烁光谱法被证明是一种快速且合适的方法,用于确定促生长和生长抑制因子对表皮细胞增殖的影响。

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