Effects of a Sertoli cell-specific knockout of Connexin43 on maturation and proliferation of postnatal Sertoli cells

IF 2.2 3区生物学 Q4 CELL BIOLOGY

Differentiation Pub Date : 2023-09-25 DOI:10.1016/j.diff.2023.09.002

Hanna Hüneke , Marion Langeheine , Kristina Rode , Klaus Jung , Adrian Pilatz , Daniela Fietz , Sabine Kliesch , Ralph Brehm

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引用次数: 0

Abstract

Adult male Sertoli cell-specific Connexin43 knockout mice (SCCx43KO) exhibit higher Sertoli cell (SC) numbers per seminiferous tubule compared to their wild type (WT) littermates. Thus, deletion of this testicular gap junction protein seems to affect the proliferative potential and differentiation of “younger” SC. Although SC have so far mostly been characterised as postmitotic cells that cease to divide and become an adult, terminally differentiated cell population at around puberty, there is rising evidence that there exist exceptions from this for a very long time accepted paradigm. Aim of this study was to investigate postnatal SC development and to figure out underlying causes for observed higher SC numbers in adult KO mice. Therefore, the amount of SC mitotic figures was compared, resulting in slightly more and prolonged detection of SC mitotic figures in KO mice compared to WT. SC counting per tubular cross section revealed significantly different time curves, and comparing proliferation rates using Bromodesoxyuridine and Sox9 showed higher proliferation rates in 8-day old KO mice. SC proliferation was further investigated by Ki67 immunohistochemistry. SC in KO mice displayed a delayed initiation of cell-cycle-inhibitor p27^Kip1 synthesis and prolonged synthesis of the phosphorylated tumour suppressor pRb and proliferation marker Ki67. Thus, the higher SC numbers in adult male SCCx43KO mice may arise due to two different reasons: Firstly, in prepubertal KO mice, the proliferation rate of SC was higher. Secondly, there were differences in their ability to cease proliferation as shown by the delayed initiation of p27^Kip1 synthesis and the prolonged production of phosphorylated pRb and Ki67. Immunohistochemical results indicating a prolonged period of SC proliferation in SCCx43KO were confirmed by detection of proliferating SC in 17-days-old KO mice. In conclusion, deletion of the testicular gap junction protein Cx43 might prevent normal SC maturation and might even alter also the proliferation potential of adult SC.

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支持细胞特异性敲除Connexin43对出生后支持细胞成熟和增殖的影响。

与野生型（WT）同窝出生的小鼠相比，成年雄性支持细胞特异性Connexin43敲除小鼠（SCCx43KO）每个曲精小管表现出更高的支持细胞（SC）数量。因此，这种睾丸间隙连接蛋白的缺失似乎会影响“年轻”SC的增殖潜力和分化。尽管到目前为止，SC大多被描述为有丝分裂后细胞，在青春期左右停止分裂并成为成年、终末分化的细胞群，越来越多的证据表明，在一个长期被接受的范式中，也存在例外。本研究的目的是研究出生后SC的发育，并找出在成年KO小鼠中观察到的SC数量较高的潜在原因。因此，比较了SC有丝分裂图的数量，导致与WT相比，KO小鼠中SC有丝裂图的检测略多且延长。每管横截面的SC计数显示出显著不同的时间曲线，并且使用溴脱氧尿苷和Sox9比较增殖率显示出8日龄KO小鼠的更高增殖率。通过Ki67免疫组化进一步研究SC的增殖。KO小鼠中的SC表现出细胞周期抑制剂p27Kip1合成的延迟启动和磷酸化肿瘤抑制因子pRb和增殖标记物Ki67的延长合成。因此，成年雄性SCCx43KO小鼠中SC数量较高可能是由于两个不同的原因：首先，在青春期前的KO小鼠中，SC的增殖率较高。其次，它们停止增殖的能力存在差异，如p27Kip1合成的延迟启动和磷酸化pRb和Ki67的延长产生所示。免疫组织化学结果表明SCCx43KO中SC增殖期延长，通过在17天大的KO小鼠中检测到增殖的SC得到证实。总之，睾丸间隙连接蛋白Cx43的缺失可能会阻止正常SC的成熟，甚至可能改变成年SC的增殖潜力。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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来源期刊

Differentiation 生物-发育生物学

CiteScore

4.10

自引率

3.40%

发文量

审稿时长

51 days

期刊介绍： Differentiation is a multidisciplinary journal dealing with topics relating to cell differentiation, development, cellular structure and function, and cancer. Differentiation of eukaryotes at the molecular level and the use of transgenic and targeted mutagenesis approaches to problems of differentiation are of particular interest to the journal. The journal will publish full-length articles containing original work in any of these areas. We will also publish reviews and commentaries on topics of current interest. The principal subject areas the journal covers are: • embryonic patterning and organogenesis • human development and congenital malformation • mechanisms of cell lineage commitment • tissue homeostasis and oncogenic transformation • establishment of cellular polarity • stem cell differentiation • cell reprogramming mechanisms • stability of the differentiated state • cell and tissue interactions in vivo and in vitro • signal transduction pathways in development and differentiation • carcinogenesis and cancer • mechanisms involved in cell growth and division especially relating to cancer • differentiation in regeneration and ageing • therapeutic applications of differentiation processes.