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针对兔肝细胞色素P-450LM2和细胞色素P-450LM4的单克隆抗体。

Monoclonal antibodies to rabbit liver cytochrome P-450LM2 and cytochrome P-450LM4.

作者信息

Park S S, Cha S J, Miller H, Persson A V, Coon M J, Gelboin H V

出版信息

Mol Pharmacol. 1982 Jan;21(1):248-58.

PMID:6813677
Abstract

Monoclonal antibodies were prepared from hybridoma clones isolated by the fusion of myeloma cells and spleen cells derived from mice immunized with either purified rabbit liver microsomal cytochrome P-450LM2 or cytochrome P-450LM4. Seven hybridoma clones produced three kinds of monoclonal antibodies to P-450LM2. The first class bound, precipitated, and inhibited the enzyme activity of P-450LM2 for both benzo[a]pyrene hydroxylation and 7-ethoxycoumarin deethylation. The other two classes either bound and precipitated or only bound the enzyme. These monoclonal antibodies to P-450LM2 showed a precipitin reaction and inhibition of enzyme activity that was specific for cytochrome P-450LM2. Thus, they did not react with or inhibit the enzyme activity of the other isozyme cytochrome P-450LM4, Fraction 1 or Fraction 7. All of the monoclonal antibodies formed against P-450LM2 were mouse immunoglobulin (Ig) subclass IgG1. The most effective monoclonal antibody strongly inhibited the formation of oxygenated metabolites of benzo[a]pyrene at various positions as well as the deethylation of 7-ethoxycoumarin. Four hybridomas were isolated which produced monoclonal antibodies to P-450LM4. One of the four was of the IgM class and three were of the IgG1 type. The four monoclonal antibodies bound to P-450LM4 but did not precipitate the enzyme, and did not bind to P-450LM2. The monoclonal antibody P-450LM4 complexes interacted with protein A, and the enzyme activity for benzo[a]pyrene hydroxylation could be removed by centrifugation. The high specificity and monoclonality of these antibodies suggest their potential usefulness for studying the genetics, regulation, and roles of the different isozymes of P-450LM in drug and carcinogen metabolism.

摘要

用纯化的兔肝微粒体细胞色素P - 450LM2或细胞色素P - 450LM4免疫小鼠,取其骨髓瘤细胞与脾细胞融合后分离得到的杂交瘤克隆制备单克隆抗体。七个杂交瘤克隆产生了三种针对P - 450LM2的单克隆抗体。第一类抗体能结合、沉淀并抑制P - 450LM2对苯并[a]芘羟基化和7 - 乙氧基香豆素脱乙基反应的酶活性。另外两类抗体要么能结合并沉淀该酶,要么仅能结合该酶。这些针对P - 450LM2的单克隆抗体表现出沉淀反应以及对细胞色素P - 450LM2特异性的酶活性抑制作用。因此,它们不与其他同工酶细胞色素P - 450LM4、组分1或组分7发生反应或抑制其酶活性。所有针对P - 450LM2形成的单克隆抗体均为小鼠免疫球蛋白(Ig)亚类IgG1。最有效的单克隆抗体强烈抑制苯并[a]芘在各个位置的氧化代谢产物的形成以及7 - 乙氧基香豆素的脱乙基反应。分离得到四个产生针对P - 450LM4单克隆抗体的杂交瘤。其中四个中的一个是IgM类,三个是IgG1类型。这四种单克隆抗体与P - 450LM4结合但不沉淀该酶,且不与P - 450LM2结合。单克隆抗体P - 450LM4复合物与蛋白A相互作用,苯并[a]芘羟基化的酶活性可通过离心去除。这些抗体的高特异性和单克隆性表明它们在研究P - 450LM不同同工酶在药物和致癌物代谢中的遗传学、调控及作用方面具有潜在用途。

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