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豚鼠肝脏Mu类谷胱甘肽S-转移酶M1-2与大鼠Mu类和theta类谷胱甘肽S-转移酶的抗体发生交叉反应。

Guinea pig liver Mu-class glutathione S-transferase M1-2 cross-reacts with antibodies to both rat Mu- and theta-class glutathione S-transferases.

作者信息

Hiratsuka A, Ogura K, Fujioka H, Sakamoto Y, Okuda H, Wada K, Tanaka T, Nishiyama T, Watabe T

机构信息

Department of Drug Metabolism and Molecular Toxicology, School of Pharmacy, Tokyo University of Pharmacy and Life Science, Japan.

出版信息

Arch Biochem Biophys. 1998 Jun 1;354(1):188-96. doi: 10.1006/abbi.1998.0649.

Abstract

Two novel major heterodimeric Mu-class glutathione (GSH) S-transferases (GSTs), designated M1-2 and M1-3*, were isolated from guinea pig (gp) liver cytosol and purified to homogeneity together with a known major homodimeric Mu-class gpGSTM1-1 (reported as GST b by R. Oshino, K. Kamei, M. Nishioka, and M. Shin, 1990, J. Biochem. 107, 105-110). These three gpGSTs were quantitatively retained on an S-hexyl-GSH affinity column and separated as homogeneous proteins by chromatofocusing. Subunits of the heterodimers were inseparable on sodium dodecyl sulfate-polyacrylamide gel electrophoresis, but could be completely separated by reverse-phase partition high-performance liquid chromatography. A molecular cloning study demonstrated that the gpGST subunit M2 consisted of 217 amino acid residues with a calculated molecular mass of 25,562 and shared 84% identity in overall amino acid sequence with gpGSTM1-1. N-terminal amino acid sequences of peptides from the gpGST subunit M3* with a blocked N-terminus strongly suggested that it should belong to the Mu class. Western blot analysis using antisera raised against purified rat (r) GSTsA1-2 (Alpha), M1-1, P1-1 (Pi), and T2-2 (Theta) indicated that gpGSTsM1-1 and M1-3* cross-reacted only with anti-rGSTM1 antibody. However, gpGSTM1-2 cross-reacted intensely to almost the same extent with antibodies to both rGSTsM1-1 and T2-2. A homodimeric gpGSTM2-2, artificially constructed from native gpGSTM1-2 by treatment with guanidine hydrochloride followed by dialysis, intensely cross-reacted with antibodies to both the rat Mu- and Theta-class GSTs. Thus, the gpGST subunit M2 provided the first evidence for the double immuno-cross-reaction of a GST with polyclonal antibodies to two different classes of GSTs.

摘要

从豚鼠肝脏胞质溶胶中分离出两种新型的主要异源二聚体 Mu 类谷胱甘肽(GSH)S-转移酶(GSTs),命名为 M1-2 和 M1-3*,并与已知的主要同源二聚体 Mu 类 gpGSTM1-1(R. Oshino、K. Kamei、M. Nishioka 和 M. Shin 在 1990 年的《生物化学杂志》107 卷,105 - 110 页报道为 GST b)一起纯化至同质。这三种 gpGSTs 被定量保留在 S-己基-GSH 亲和柱上,并通过色谱聚焦作为同质蛋白质分离。异源二聚体的亚基在十二烷基硫酸钠-聚丙烯酰胺凝胶电泳上不可分离,但可通过反相分配高效液相色谱完全分离。一项分子克隆研究表明,gpGST 亚基 M2 由 217 个氨基酸残基组成,计算分子量为 25,562,在整体氨基酸序列上与 gpGSTM1-1 具有 84%的同一性。来自 gpGST 亚基 M3的 N 端被封闭的肽段的 N 端氨基酸序列强烈表明它应属于 Mu 类。使用针对纯化的大鼠(r)GSTsA1-2(Alpha)、M1-1、P1-1(Pi)和 T2-2(Theta)产生的抗血清进行的 Western 印迹分析表明,gpGSTsM1-1 和 M1-3仅与抗 rGSTM1 抗体发生交叉反应。然而,gpGSTM1-2 与抗 rGSTsM1-1 和 T2-2 的抗体几乎以相同程度强烈交叉反应。通过用盐酸胍处理天然 gpGSTM1-2 然后透析人工构建的同源二聚体 gpGSTM2-2 与大鼠 Mu 类和 Theta 类 GSTs 的抗体都强烈交叉反应。因此,gpGST 亚基 M2 首次证明了一种 GST 与针对两种不同类 GSTs 的多克隆抗体发生双重免疫交叉反应。

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