具有组织蛋白酶D活性的蚊子溶酶体天冬氨酸蛋白酶的纯化与鉴定

Wen-Long Cho, Tarlochan S. Dhadialla, Alexander S. Raikhel
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引用次数: 28

摘要

从埃及伊蚊中纯化并鉴定了一种具有组织蛋白酶D活性的溶酶体天冬氨酸蛋白酶。采用硫酸铵(30-50%)和酸(pH 2.5)沉淀法从全蚊中提取蛋白质,然后用阳离子交换色谱法分离。用SDS-PAGE和银染色法检测酶的纯度。在非变性条件下,聚丙烯酰胺凝胶电泳测定纯化酶的天然分子量为80,000。SDS-PAGE将酶分解为单个多肽,Mr = 40000,表明它在非变性状态下以同型二聚体存在。经等电聚焦凝胶电泳测定,纯化酶的pI为5.4。纯化后的酶具有组织蛋白酶d的特性,它利用血红蛋白作为底物,其活性被胃抑素- a和6M尿素完全抑制,但不受10 mM KCN的抑制。纯化后的天冬氨酸蛋白酶在pH 3.0和45℃条件下活性最佳。以血红蛋白为底物,酶的表观Km为4.2 μ m,在家兔中制备了对纯化酶的多克隆抗体。通过对蚊子粗提取物和非变性酶及SDS-PAGE分离酶的免疫印迹分析,验证了抗体对该酶的特异性。对细胞器进行密度梯度离心,然后进行酶和免疫印迹分析,证实了纯化酶的溶酶体性质。纯化的蚊子溶酶体蛋白酶n端氨基酸序列(19个氨基酸)与猪和人组织蛋白酶D n端氨基酸序列同源性达74%。
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Purification and characterization of a lysosomal aspartic protease with cathepsin D activity from the mosquito

A lysosomal aspartic protease with cathepsin D activity, from the mosquito, Aedes aegypti, was purified and characterized. Its isolation involved ammonium sulfate (30–50%) and acid (pH 2.5) precipitations of protein extracts from whole previtellogenic mosquitoes followed by cation exchange chromatography. Purity of the enzyme was monitored by SDS-PAGE and silver staining of the gels. The native molecular weight of the purified enzyme as determined by polyacrylamide gel electrophoresis under nondenaturing conditions was 80,000. SDS-PAGE resolved the enzyme into a single polypeptide with Mr = 40,000 suggesting that it exists as a homodimer in its non-denatured state. The pI of the purified enzyme was 5.4 as determined by isoelectric focusing gel electrophoresis. The purified enzyme exhibits properties characteristic of cathepsin D. It utilizes hemoglobin as a substrate and its activity is completely inhibited by pepstatin-A and 6M urea but not by 10 mM KCN. Optimal activity of the purified mosquito aspartic protease was obtained at pH 3.0 and 45°C. With hemoglobin as a substrate the enzyme had an apparent Km of 4.2 μ M. Polyclonal antibodies to the purified enzyme were raised in rabbits. The specificity of the antibodies to the enzyme was verified by immunoblot analysis of crude mosquito extracts and the enzyme separated by both non-denaturing and SDS-PAGE. Density gradient centrifugation of organelles followed by enzymatic and immunoblot analyses demonstrated the lysosomal nature of the purified enzyme. The N-terminal amino acid sequence of the purified mosquito lysosomal protease (19 amino acids) has 74% identity with N-terminal amino acid sequence of porcine and human cathepsins D.

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