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在终末分化的鸡晶状体纤维中,各种基因对内源DNA酶活性的敏感性增加。

Increased sensitivity of various genes to endogenous DNase activity in terminal differentiating chick lens fibers.

作者信息

Muel A S, Laurent M, Chaudun E, Alterio J, Clayton R, Courtois Y, Counis M F

机构信息

Unité de Recherches Gérontologiques, U 118 INSERM, Paris, France.

出版信息

Mutat Res. 1989 May;219(3):157-64. doi: 10.1016/0921-8734(89)90010-6.

DOI:10.1016/0921-8734(89)90010-6
PMID:2739672
Abstract

In the lens, epithelial cells from the equatorial zone differentiate into postmitotic elongated fibers. One aspect of this differentiation is nuclear shape transformation and DNA degradation. This process is controlled by DNase activity which in fiber nuclei increases with development. DNase activity is also present in the epithelial cell nuclei which appears to be non-functional but could be activated in vitro by exogenous addition of Ca2+. We have analyzed the possible selective action of endogenous DNase on 3 genes involved in lens terminal differentiation, namely delta-crystallin, beta-tubulin and vimentin, and on 1 gene not thought to participate in this process, ovalbumin. We have compared restriction DNA patterns of these genes in nuclei isolated from 11-day-old chick embryos and incubated in Ca2+-free medium or in fresh epithelial and fiber lens tissue at 11 and 18 days of development. During incubation in vitro of 11-day fiber nuclei, there is a net increase in the sensitivity of the delta-crystallin, beta-tubulin, ovalbumin and vimentin chromatin to the endogenous DNase. The vimentin gene appears to be more stable than the beta-tubulin and delta-crystallin genes indicating a degree of specificity of the endogenous DNase activity. In the epithelial nuclei, the lens-specific genes appear to be more stable but paradoxically there is a net degradation of the ovalbumin gene. In freshly isolated tissues the 4 genes were detected in epithelial and fiber cells at 11 and 18 days. Furthermore, in the mature fibers in which the nuclei were degenerating, the latter genes were still not completely digested.

摘要

在晶状体中,赤道区的上皮细胞分化为有丝分裂后伸长的纤维。这种分化的一个方面是核形状转变和DNA降解。该过程由DNase活性控制,其在纤维核中的活性随发育而增加。DNase活性也存在于上皮细胞核中,上皮细胞核中的DNase活性似乎没有功能,但在体外通过外源添加Ca2+可被激活。我们分析了内源性DNase对晶状体终末分化涉及的3个基因(即δ-晶状体蛋白、β-微管蛋白和波形蛋白)以及1个被认为不参与此过程的基因(卵清蛋白)可能的选择性作用。我们比较了从11日龄鸡胚分离的细胞核以及在发育11天和18天时在无Ca2+培养基或新鲜的上皮和纤维晶状体组织中孵育后的这些基因的限制性DNA图谱。在体外孵育11日龄的纤维核时,δ-晶状体蛋白、β-微管蛋白、卵清蛋白和波形蛋白染色质对内源性DNase的敏感性净增加。波形蛋白基因似乎比β-微管蛋白和δ-晶状体蛋白基因更稳定,表明内源性DNase活性具有一定程度的特异性。在上皮细胞核中,晶状体特异性基因似乎更稳定,但矛盾的是卵清蛋白基因有净降解。在新鲜分离的组织中,在发育11天和18天时在上皮细胞和纤维细胞中检测到这4个基因。此外,在核正在退化的成熟纤维中,后几个基因仍未被完全消化。

相似文献

1
Increased sensitivity of various genes to endogenous DNase activity in terminal differentiating chick lens fibers.在终末分化的鸡晶状体纤维中,各种基因对内源DNA酶活性的敏感性增加。
Mutat Res. 1989 May;219(3):157-64. doi: 10.1016/0921-8734(89)90010-6.
2
Nuclear endogenous Ca2+-dependent endodeoxyribonuclease in differentiating chick embryonic lens fibers.分化中的鸡胚晶状体纤维中的细胞核内源性钙依赖性内切脱氧核糖核酸酶
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Curr Eye Res. 1987 Nov;6(11):1275-81. doi: 10.3109/02713688708997552.
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DNAase activities in embryonic chicken lens: in epithelial cells or in differentiating fibers where chromatin is progressively cleaved.
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Involvement of DNase II in nuclear degeneration during lens cell differentiation.脱氧核糖核酸酶II在晶状体细胞分化过程中参与细胞核退化。
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Reiteration frequency of delta-crystallin DNA in lens and non-lens tissues of chick embryos. delta-Crystallin gene is not amplified during lens cell differentiation.鸡胚晶状体和非晶状体组织中δ-晶状体蛋白DNA的重复频率。在晶状体细胞分化过程中,δ-晶状体蛋白基因未被扩增。
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The pattern of expression of chick delta-crystallin genes in lens differentiation and in trans-differentiating cultured tissues.鸡δ-晶体蛋白基因在晶状体分化及培养组织转分化过程中的表达模式。
EMBO J. 1983;2(3):333-8. doi: 10.1002/j.1460-2075.1983.tb01427.x.

引用本文的文献

1
Chromatin degradation in differentiating fiber cells of the eye lens.眼晶状体分化纤维细胞中的染色质降解。
J Cell Biol. 1997 Apr 7;137(1):37-49. doi: 10.1083/jcb.137.1.37.
2
Decrease of DNA per cell during development of the lens in chickens.
Histochemistry. 1990;94(3):293-6. doi: 10.1007/BF00266630.