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在人胎盘中鉴定出一种Mg2+依赖性蛋白酶,该酶可将疏水性叶酸结合蛋白切割成亲水性形式。

Identification of a Mg2+-dependent protease in human placenta which cleaves hydrophobic folate-binding proteins to hydrophilic forms.

作者信息

Antony A C, Verma R S, Unune A R, LaRosa J A

机构信息

Department of Medicine, Indiana University School of Medicine, Indianapolis 46223.

出版信息

J Biol Chem. 1989 Feb 5;264(4):1911-4.

PMID:2536692
Abstract

Hydrophobic folate-binding proteins (FBPs), which are only 5-10 kDa larger than 40-kDa hydrophilic FBPs, bind significant quantities of Triton X-100 micelles and elute as apparent 160-kDa species on Sephacryl S-200 gel filtration in Triton X-100. Detergent-solubilized placental membranes release a major (greater than 95%) 40-kDa hydrophilic FBP species as well as a minor apparent 160-kDa folate binding species when similarly analyzed. We tested the hypothesis that this recovery of predominantly hydrophilic FBPs was mediated by a putative hydrophobic FBP-specific placental protease. When placenta was solubilized in the presence of increasing concentrations of EDTA, there was a progressive increase in apparent 160-kDa folate binding moieties concomitant with a decrease in 40-kDa FBPs. At 20 mM EDTA, a single apparent 160-kDa folate binding species was recovered and the 40-kDa FBPs could not be detected by radioligand binding or specific radioimmunoassay. The apparent 160-kDa species specifically bound radiolabeled folates and were specifically immunoprecipitated by rabbit anti-40-kDa FBP antiserum. On 15% sodium dodecyl sulfate-polyacrylamide gel electrophoresis followed by transfer to nitrocellulose and probing with anti-40-kDa FBP antiserum, the apparent 160-kDa FBPs electrophoresed as 45-kDa species. Detergent binding studies indicated that apparent 160-kDa FBPs were hydrophobic, thus accounting for the molecular weight discrepancy in gel filtration in Triton X-100 versus sodium dodecyl sulfate-polyacrylamide gel electrophoresis. The EDTA-mediated inhibition of conversion of hydrophobic FBPs to hydrophilic FBPs by protease was reversed in a dose-dependent manner by Mg2+. If this protease is physiologically relevant, it could play an important regulatory role in folate transport by influencing the net number of hydrophobic FBPs on the cell surface.

摘要

疏水叶酸结合蛋白(FBP)比40 kDa的亲水FBP仅大5 - 10 kDa,能结合大量Triton X - 100胶束,并在含Triton X - 100的Sephacryl S - 200凝胶过滤中以表观160 kDa的形式洗脱。当对去污剂溶解的胎盘膜进行类似分析时,会释放出一种主要的(超过95%)40 kDa亲水FBP以及一种次要的表观160 kDa叶酸结合物质。我们检验了这样一个假设,即这种主要为亲水FBP的回收是由一种假定的疏水FBP特异性胎盘蛋白酶介导的。当胎盘在浓度不断增加的EDTA存在下溶解时,表观160 kDa叶酸结合部分逐渐增加,同时40 kDa FBP减少。在20 mM EDTA时,回收了单一的表观160 kDa叶酸结合物质,通过放射性配体结合或特异性放射免疫测定法无法检测到40 kDa FBP。表观160 kDa物质特异性结合放射性标记的叶酸,并被兔抗40 kDa FBP抗血清特异性免疫沉淀。在15%十二烷基硫酸钠 - 聚丙烯酰胺凝胶电泳后转移至硝酸纤维素膜并用抗40 kDa FBP抗血清进行检测时,表观160 kDa FBP电泳显示为45 kDa物质。去污剂结合研究表明表观160 kDa FBP是疏水的,这解释了在Triton X - 100中的凝胶过滤与十二烷基硫酸钠 - 聚丙烯酰胺凝胶电泳之间分子量的差异。Mg2+以剂量依赖的方式逆转了EDTA介导的蛋白酶对疏水FBP向亲水FBP转化的抑制作用。如果这种蛋白酶具有生理相关性,它可能通过影响细胞表面疏水FBP的净数量在叶酸转运中发挥重要的调节作用。

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