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一种T细胞杂交瘤产生的单克隆非特异性抑制因子(MNSF)的分离与鉴定。

Isolation and characterization of a monoclonal nonspecific suppressor factor (MNSF) produced by a T cell hybridoma.

作者信息

Nakamura M, Ogawa H, Tsunematsu T

出版信息

J Immunol. 1986 Apr 15;136(8):2904-9.

PMID:2420877
Abstract

By fusing Con A-activated BALB/c mice spleen cells with AKR thymoma BW5147 cells, we prepared a hybridoma producing a monoclonal nonspecific suppressor factor (MNSF). This factor inhibits a generation of LPS-induced immunoglobulin-secreting cells. We used ELISA for the bioassay of MNSF activity. With this method, a stable E17 hybridoma clone was selected, and its product in culture medium was isolated and characterized. MNSF fractionated on Sephadex G-100 in saline buffer shows a form with multiple m.w., but fractionated in 0.4 M pyridine-acetic buffer, it is limited to two species of approximately 24Kd and 16Kd. The MNSF was purified by hydroxyapatite chromatography, with marked effectiveness. MNSF activity was found exclusively in the 0.35 M sodium phosphate elution, and the content was further fractionated on subsequent gel filtration in the high ionic strength buffer described above. The purified factor exhibited two forms, of 24Kd and 16Kd, and showed peaks of pI 5.3 and 5.7, respectively, on isoelectric focusing. The MNSF preparation described here is stable at 56 degrees C and unaffected by 2-mercaptoethanol, but is unstable at pH 2.0 and is sensitive to tryptic proteolysis. We injected the hybridoma cells into the peritoneal cavity of pristane-primed F1 (AKR/J X BALB/c) mice, and a large amount of pure MNSF was obtained from the ascites, the characteristics of which were similar to those in the culture supernatant. Thus, the MNSF obtained from the E17 hybridoma consists of functionally identical but physicochemically different discrete proteins. This simple method of purification can serve as a probe for further characterization of MNSF and its application in in vivo experiments.

摘要

通过将刀豆蛋白A激活的BALB/c小鼠脾细胞与AKR胸腺瘤BW5147细胞融合,我们制备了一种产生单克隆非特异性抑制因子(MNSF)的杂交瘤。该因子可抑制脂多糖诱导的免疫球蛋白分泌细胞的产生。我们使用酶联免疫吸附测定法(ELISA)对MNSF活性进行生物测定。通过这种方法,筛选出了稳定的E17杂交瘤克隆,并对其培养基中的产物进行了分离和鉴定。在盐缓冲液中经葡聚糖凝胶G-100分级分离的MNSF呈现出多种分子量形式,但在0.4M吡啶-乙酸缓冲液中分级分离时,它仅限于两种约24Kd和16Kd的形式。MNSF通过羟基磷灰石色谱法进行纯化,效果显著。MNSF活性仅在0.35M磷酸钠洗脱液中被发现,其含量在随后上述高离子强度缓冲液中的凝胶过滤中进一步分级分离。纯化后的因子呈现出24Kd和16Kd两种形式,在等电聚焦时分别显示出pI 5.3和5.7的峰。这里描述的MNSF制剂在56℃下稳定,不受2-巯基乙醇影响,但在pH 2.0时不稳定,对胰蛋白酶水解敏感。我们将杂交瘤细胞注入经 pristane 预处理的F1(AKR/J×BALB/c)小鼠的腹腔中,从腹水中获得了大量纯MNSF,其特性与培养上清液中的相似。因此,从E17杂交瘤获得的MNSF由功能相同但物理化学性质不同的离散蛋白质组成。这种简单的纯化方法可作为进一步鉴定MNSF及其在体内实验中应用的探针。

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J Immunol. 1986 Apr 15;136(8):2904-9.
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