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海胆芳基硫酸酯酶基因的结构及组织特异性发育表达

Structure and tissue-specific developmental expression of a sea urchin arylsulfatase gene.

作者信息

Yang Q, Angerer L M, Angerer R C

机构信息

Department of Biology, University of Rochester, New York 14627.

出版信息

Dev Biol. 1989 Sep;135(1):53-65. doi: 10.1016/0012-1606(89)90157-7.

DOI:10.1016/0012-1606(89)90157-7
PMID:2767335
Abstract

Arylsulfatases are a group of enzymes that remove sulfate moieties from a diverse set of substrates including glycoproteins, steroids, and cerebrosides. We have isolated recombinant cDNA clones corresponding to an arylsulfatase (SpARS) message that encodes an abundant protein of pluteus larvae of the sea urchin Strongylocentrotus purpuratus. Although vertebrate arylsulfatases have broad tissue distributions, in situ hybridization with a probe for SpARS shows that the sea urchin message accumulates in the embryo only in the single cell type of aboral ectoderm and its precursors. The message is first detectable by RNase protection assays around hatching blastula stage and accumulates through pluteus larva stage. The open reading frame of cDNA clones is 1701 nt long and encodes a deduced protein with a predicted molecular mass of 61 kDa. Analysis of corresponding genomic DNA clones reveals that the pre-mRNA contains six exons. Consistent with the fact that arylsulfatase enzyme activity is extracellular, this polypeptide has a hydrophobic leader sequence and three potential glycosylation sites. Furthermore, hybridization in situ shows that in blastulae arylsulfatase message is preferentially concentrated around nuclei at the basal sides of cells. The S. purpuratus sequence is very similar to that recently reported for the same enzyme from Hemicentrotus pulcherrimus and 30% of the amino acid residues are also identical to those of both human arylsulfatase C (steroid sulfatase) and arylsulfatase A. Sequence relationships among these four mRNAs suggest that, assuming equal rates of evolution, the duplication separating the human genes occurred at about the time of separation of the echinoderm and vertebrate lineages.

摘要

芳基硫酸酯酶是一组能从多种底物(包括糖蛋白、类固醇和脑苷脂)上移除硫酸基团的酶。我们已分离出与一种芳基硫酸酯酶(SpARS)信使核糖核酸(mRNA)相对应的重组互补脱氧核糖核酸(cDNA)克隆,该信使核糖核酸编码紫海胆强壮柱头虫幼虫中一种丰富的蛋白质。尽管脊椎动物的芳基硫酸酯酶具有广泛的组织分布,但用SpARS探针进行的原位杂交显示,海胆的信使核糖核酸仅在口外胚层及其前体的单一细胞类型中在胚胎中积累。通过核糖核酸酶保护分析,在孵化囊胚期左右首次可检测到该信使核糖核酸,并且在长腕幼虫期积累。cDNA克隆的开放阅读框长1701个核苷酸,编码一种推导的蛋白质,预测分子量为61 kDa。对相应基因组DNA克隆的分析表明,前体信使核糖核酸包含六个外显子。与芳基硫酸酯酶的酶活性是细胞外的这一事实一致,该多肽具有一个疏水前导序列和三个潜在的糖基化位点。此外,原位杂交显示,在囊胚中,芳基硫酸酯酶信使核糖核酸优先集中在细胞基部一侧的细胞核周围。紫海胆的序列与最近报道的来自美丽海胆的同一种酶的序列非常相似,并且30%的氨基酸残基也与人类芳基硫酸酯酶C(类固醇硫酸酯酶)和芳基硫酸酯酶A的相同。这四种信使核糖核酸之间的序列关系表明,假设进化速率相等,将人类基因分开的复制大约发生在棘皮动物和脊椎动物谱系分离之时。

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