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不动杆菌和大肠杆菌脂多糖制剂对成年和新生猪淋巴细胞的比较促有丝分裂活性及体外免疫球蛋白合成诱导作用

Acinetobacter and E. coli lipopolysaccharide preparations comparative mitogenicity and induction in vitro of immunoglobulin synthesis in adult and neonatal pig lymphocytes.

作者信息

Symons D B, Clarkson C A

出版信息

Immunology. 1979 Nov;38(3):601-7.

Abstract

Lipopolysaccharide (LPS) was prepared by phenol/water extraction of bacterial membranes prepared from Acinetobacter and Escherichia coli. The mitogenicity of laboratory-prepared LPS was significantly greater than that of commercial E. coli LPS for pig, sheep, calf and rat lymphocytes, assayed as [3H]-thymidine incorporation. Mouse lymphocytes responded well to commercial LPS and no greater response was obtained with other LPS preparations. A small proportion (14%) of the Acinetobacter LPS preparations was soluble in aqueous medium, the remainder comprising membraneous fragments of variable form and size. It is suggested that the insoluble presentation of LPS to cells may contribute to the improved mitogenicity compared with wholly soluble LPS. Acinetobacter LPS preparations were used to induce synthesis and secretion in vitro of immunoglobulin by adult blood lymphocytes and pre-suckled, neonatal spleen cells of the pig. IgM was the dominant class of immunoglobulin secreted. This work thus demonstrated that virgin, unprimed B cells could be induced into immunoglobulin secretion by mitogen stimulation.

摘要

脂多糖(LPS)通过苯酚/水萃取法从不动杆菌和大肠杆菌制备的细菌膜中提取。以[3H] - 胸腺嘧啶核苷掺入量测定,实验室制备的LPS对猪、羊、小牛和大鼠淋巴细胞的促有丝分裂活性明显高于市售大肠杆菌LPS。小鼠淋巴细胞对市售LPS反应良好,其他LPS制剂未获得更大反应。一小部分(14%)不动杆菌LPS制剂可溶于水性介质,其余部分由形态和大小各异的膜碎片组成。有人认为,与完全可溶的LPS相比,LPS以不溶性形式呈现给细胞可能有助于提高其促有丝分裂活性。不动杆菌LPS制剂用于诱导成年猪血液淋巴细胞和仔猪吮乳前的新生脾细胞体外合成和分泌免疫球蛋白。IgM是分泌的主要免疫球蛋白类别。因此,这项工作表明,未接触过抗原的原始B细胞可通过有丝分裂原刺激诱导分泌免疫球蛋白。

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A new method for the extraction of R lipopolysaccharides.一种提取R脂多糖的新方法。
Eur J Biochem. 1969 Jun;9(2):245-9. doi: 10.1111/j.1432-1033.1969.tb00601.x.
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Interaction of lipopolysaccharides and lipid A with complement.脂多糖和脂质A与补体的相互作用。
Eur J Biochem. 1971 Mar 1;19(1):143-52. doi: 10.1111/j.1432-1033.1971.tb01298.x.

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