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使用表皮聚丝蛋白 cDNA 所证实的聚丝蛋白基因的重复结构。

The repetitive structure of the profilaggrin gene as demonstrated using epidermal profilaggrin cDNA.

作者信息

Haydock P V, Dale B A

出版信息

J Biol Chem. 1986 Sep 25;261(27):12520-5.

PMID:3755723
Abstract

Filaggrin is the histidine-rich basic protein that aggregates keratin filaments in fully differentiated cells of the epidermis. Filaggrin is synthesized in the granular cell layer as a high molecular weight precursor protein (profilaggrin) that consists of multiple repeated copies of filaggrin. cDNA clones for rat and mouse epidermal profilaggrin have been constructed from sucrose gradient-enriched RNA in order to study the repetitive structure of profilaggrin. These clones hybridize to high molecular weight epidermal mRNA (23 kilobase pairs, rat and 19 kilobase pairs, mouse) and exhibit limited cross-hybridization between species. Several rat clones direct the synthesis of a portion of rat profilaggrin in bacteria. One of these, rat profilaggrin cDNA clone R4D6, is 2400 base pairs in length. The R4D6 cDNA is shown to contain repetitive sequence by restriction mapping and southern hybridization analysis of restriction digests of this plasmid, using subfragments of the plasmid as hybridization probes. Southern hybridization analysis of rat genomic DNA, digested to completion with several restriction enzymes, reveals a simple hybridization pattern of fragments equal in size to those of the cDNA. Partial digestion of rat genomic DNA results in a ladder of bands based on a 1200-base pair repeat, equal to the size of the repeating unit of the cDNA clone, and consistent with the expected repeating size of profilaggrin. Together, these results show that the profilaggrin mRNA and gene have repetitive structure and that the gene apparently lacks introns in the coding region.

摘要

丝聚合蛋白是一种富含组氨酸的碱性蛋白,它能使表皮完全分化细胞中的角蛋白丝聚集。丝聚合蛋白在颗粒层细胞中作为一种高分子量前体蛋白(前丝聚合蛋白)合成,前丝聚合蛋白由多个丝聚合蛋白重复拷贝组成。为了研究前丝聚合蛋白的重复结构,已从蔗糖梯度富集的RNA构建了大鼠和小鼠表皮前丝聚合蛋白的cDNA克隆。这些克隆与高分子量表皮mRNA(大鼠为23千碱基对,小鼠为19千碱基对)杂交,并且在种间表现出有限的交叉杂交。几个大鼠克隆可指导细菌中大鼠部分前丝聚合蛋白的合成。其中一个,大鼠前丝聚合蛋白cDNA克隆R4D6,长度为2400个碱基对。通过对该质粒的限制性酶切图谱分析以及使用该质粒的亚片段作为杂交探针进行Southern杂交分析,表明R4D6 cDNA含有重复序列。用几种限制性酶完全消化大鼠基因组DNA后的Southern杂交分析显示,片段的杂交模式简单,其大小与cDNA的片段相等。大鼠基因组DNA的部分消化产生了一个基于1200碱基对重复的条带阶梯,这与cDNA克隆的重复单元大小相等,并且与预期的前丝聚合蛋白重复大小一致。这些结果共同表明,前丝聚合蛋白mRNA和基因具有重复结构,并且该基因在编码区域显然缺乏内含子。

相似文献

1
The repetitive structure of the profilaggrin gene as demonstrated using epidermal profilaggrin cDNA.使用表皮聚丝蛋白 cDNA 所证实的聚丝蛋白基因的重复结构。
J Biol Chem. 1986 Sep 25;261(27):12520-5.
2
Filaggrin, an intermediate filament-associated protein: structural and functional implications from the sequence of a cDNA from rat.丝聚合蛋白,一种中间丝相关蛋白:来自大鼠的cDNA序列的结构和功能意义
DNA Cell Biol. 1990 May;9(4):251-61. doi: 10.1089/dna.1990.9.251.
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The gene for mouse epidermal filaggrin precursor. Its partial characterization, expression, and sequence of a repeating filaggrin unit.小鼠表皮聚角蛋白微丝蛋白前体基因。其部分特征、表达及聚角蛋白微丝蛋白重复单元的序列。
J Biol Chem. 1987 Nov 15;262(32):15643-8.
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Characterization of the human epidermal profilaggrin gene. Genomic organization and identification of an S-100-like calcium binding domain at the amino terminus.人类表皮聚丝蛋白基因的特征分析。基因组结构及氨基末端S-100样钙结合结构域的鉴定。
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Multiple copies of phosphorylated filaggrin in epidermal profilaggrin demonstrated by analysis of tryptic peptides.通过胰蛋白酶肽段分析证实表皮前丝聚合蛋白中存在多个磷酸化丝聚合蛋白拷贝。
Biochemistry. 1985 Jul 16;24(15):4167-75. doi: 10.1021/bi00336a053.
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Characterization of mouse profilaggrin: evidence for nuclear engulfment and translocation of the profilaggrin B-domain during epidermal differentiation.小鼠兜甲蛋白原的特性:表皮分化过程中兜甲蛋白原B结构域的核内吞噬及易位证据
J Invest Dermatol. 2002 Oct;119(4):905-12. doi: 10.1046/j.1523-1747.2002.00133.x.
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Evidence for specific proteolytic cleavage of the N-terminal domain of human profilaggrin during epidermal differentiation.在表皮分化过程中人类原聚角蛋白中间丝相关蛋白N端结构域发生特异性蛋白水解切割的证据。
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Characterization of protease processing sites during conversion of rat profilaggrin to filaggrin.大鼠前丝聚合蛋白转化为丝聚合蛋白过程中蛋白酶切割位点的鉴定
Biochemistry. 1993 Sep 28;32(38):10036-45. doi: 10.1021/bi00089a020.

引用本文的文献

1
The Discovery and Function of Filaggrin.丝聚合蛋白的发现与功能。
Int J Mol Sci. 2022 Jan 27;23(3):1455. doi: 10.3390/ijms23031455.
2
Optimization of filaggrin expression and processing in cultured rat keratinocytes.培养的大鼠角质形成细胞中丝聚蛋白的表达和处理的优化。
J Dermatol Sci. 2011 Jan;61(1):51-9. doi: 10.1016/j.jdermsci.2010.11.003. Epub 2010 Nov 13.
3
Characterisation of the rat oesophagus epithelium antigens defined by the so-called 'antikeratin antibodies', specific for rheumatoid arthritis.由类风湿性关节炎特异性的所谓“抗角蛋白抗体”所定义的大鼠食管上皮抗原的特性分析。
Ann Rheum Dis. 1993 Oct;52(10):749-57. doi: 10.1136/ard.52.10.749.
4
Characterization of a cDNA clone encoding human filaggrin and localization of the gene to chromosome region 1q21.编码人丝聚合蛋白的cDNA克隆的特性鉴定及该基因在染色体1q21区域的定位
Proc Natl Acad Sci U S A. 1989 Jul;86(13):4848-52. doi: 10.1073/pnas.86.13.4848.
5
Keratohyalin granules are heterogeneous in ridged and non-ridged human skin: evidence from anti-filaggrin immunogold labelling of normal skin and skin of autosomal dominant ichthyosis vulgaris patients.角蛋白透明颗粒在有嵴和无嵴的人类皮肤中具有异质性:来自正常皮肤和常染色体显性寻常型鱼鳞病患者皮肤的抗丝聚蛋白免疫金标记证据。
Arch Dermatol Res. 1991;283(7):421-32. doi: 10.1007/BF00371777.
6
The expression of skin-specific gene K51 in the epidermal layer of human skin and in basal cell carcinoma cells.皮肤特异性基因K51在人皮肤表皮层及基底细胞癌细胞中的表达。
Arch Dermatol Res. 1991;283(2):113-8. doi: 10.1007/BF00371619.