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在转基因小鼠乳汁中产生活性抗CD6小鼠/人嵌合抗体。

Production of active anti-CD6 mouse/human chimeric antibodies in the milk of transgenic mice.

作者信息

Limonta J, Pedraza A, Rodríguez A, Freyre F M, Barral A M, Castro F O, Lleonart R, Gracía C A, Gavilondo J V, de la Fuente J

机构信息

Mammalian Cell Genetics Division, Center for Genetic Engineering and Biotechnology, Havana, Cuba.

出版信息

Immunotechnology. 1995 Aug;1(2):107-13. doi: 10.1016/1380-2933(95)00010-0.

DOI:10.1016/1380-2933(95)00010-0
PMID:9373339
Abstract

The expression of chimeric genes in the mammary gland of transgenic farm animals has become an alternative for the large-scale production of recombinant proteins and for the modification of milk composition. In this paper, we show that a mouse/human chimeric antibody against the human CD6 leukocyte antigen can be assembled and correctly folded by the mammary gland, and secreted to milk, where it maintains its specificity. The base sequences encoding for the heavy and light chain variable regions of the anti-CD6 mouse monoclonal antibody IOR-T1 were cloned by the polymerase chain reaction from hybridoma cDNA, coupled to human heavy and light chain constant region genes, and inserted in a vector containing the 5' regulatory region of the rabbit whey acidic protein gene. Transgenic mice were produced by conventional pronuclei microinjection techniques. Integration and transgene copy number were determined by Southern blot. Assembled human immunoglobulin was detected in milk using a sandwich ELISA. Expression levels of chimeric antibodies in milk were determined to be around 400 micrograms/ml by Western blot, using CHO-derived chimeric IOR-T1 antibodies as reference. The chimeric antibodies produced in milk recognized human peripheral blood T lymphocytes by indirect immunofluorescence, with the classical patch-like pattern of IOR-T1.

摘要

在转基因农场动物的乳腺中表达嵌合基因,已成为大规模生产重组蛋白以及改变牛奶成分的一种替代方法。在本文中,我们展示了一种针对人CD6白细胞抗原的小鼠/人嵌合抗体能够在乳腺中组装并正确折叠,然后分泌到乳汁中,并在乳汁中保持其特异性。通过聚合酶链反应从杂交瘤cDNA中克隆出编码抗CD6小鼠单克隆抗体IOR-T1重链和轻链可变区的碱基序列,将其与人重链和轻链恒定区基因偶联,并插入到含有兔乳清酸性蛋白基因5'调控区的载体中。通过传统的原核显微注射技术制备转基因小鼠。通过Southern印迹法确定整合情况和转基因拷贝数。使用夹心ELISA在乳汁中检测组装好的人免疫球蛋白。以CHO来源的嵌合IOR-T1抗体为参照,通过Western印迹法测定乳汁中嵌合抗体的表达水平约为400微克/毫升。乳汁中产生的嵌合抗体通过间接免疫荧光法识别人类外周血T淋巴细胞,呈现出IOR-T1典型的斑块状模式。

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