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从天然来源中分离和纯化趋化因子。

Isolation and purification of chemokines from natural sources.

作者信息

Schröder J M

机构信息

Department of Dermatology, University of Kiel, D-24105 Kiel, Germany.

出版信息

Mol Biotechnol. 2001 May;18(1):71-7. doi: 10.1385/MB:18:1:71.

Abstract

Chemokines (e.g., IL-8) were originally identified as chemotactic proteins obtained from various different natural sources. Today, using the genome walking strategy an ever-increasing number of novel genes encoding chemokines have been discovered that were expressed in bacteria or eukaryotic cells and subsequently tested for biological activity. Usually biological significance of the considered chemokine is extrapolated from these data. The increasing evidence, however, that post-translational modification of chemokines can dramatically affect its biological activity makes it necessary to identify the naturally occurring chemokines in order to identify its biological function. Furthermore, with the isolation of natural chemokines, evidence is provided that transcription of chemokine genes is really followed by translation into a bioactive molecule. Purification of chemokines from natural sources requires special strategies: The bioassay or immunoassay should allow screening of high-performance liquid chromatography fractions and detection of the required chemokine at low concentration. Parameters that affect the detection of bioactivity and immunoreactivity (giving either false positive or false negative results) should be carefully considered. In this article methods for molecular characterization of chemokines from both cell culture supernatants and human tissue (lesional inflammatory skin scales) will be described.

摘要

趋化因子(如白细胞介素-8)最初被鉴定为从各种不同天然来源获得的趋化蛋白。如今,通过基因组步移策略,已发现越来越多编码趋化因子的新基因,这些基因在细菌或真核细胞中表达,随后对其生物活性进行检测。通常,所考虑趋化因子的生物学意义是从这些数据推断出来的。然而,越来越多的证据表明,趋化因子的翻译后修饰可显著影响其生物活性,这使得有必要鉴定天然存在的趋化因子,以便确定其生物学功能。此外,随着天然趋化因子的分离,有证据表明趋化因子基因的转录确实会接着翻译为生物活性分子。从天然来源纯化趋化因子需要特殊策略:生物测定或免疫测定应允许筛选高效液相色谱馏分,并在低浓度下检测所需的趋化因子。应仔细考虑影响生物活性和免疫反应性检测(产生假阳性或假阴性结果)的参数。本文将描述从细胞培养上清液和人体组织(病变炎性皮肤鳞屑)中对趋化因子进行分子表征的方法。

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