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培养的人单核细胞分泌的补体亚成分C1q具有与血清C1q相同的亚基结构。

Complement subcomponent C1q secreted by cultured human monocytes has subunit structure identical with that of serum C1q.

作者信息

Tenner A J, Volkin D B

出版信息

Biochem J. 1986 Jan 15;233(2):451-8. doi: 10.1042/bj2330451.

Abstract

An enzyme-linked immunosorbent assay (e.l.i.s.a.) that is capable of quantifying C1q concentrations as low as 2 ng/ml and a sensitive haemolytic assay were used to study the appearance of material that cross-reacts with human serum C1q as well as C1q haemolytic activity in human monocyte culture media. This material was detected in the medium after 10-14 days and continued to be secreted through to day 28 of culture, at which time the cultures were terminated. Material specifically immunoabsorbed with Sepharose-anti-C1q antibody from a culture medium of cells that was metabolically labelled with [3H] proline or [35S] methionine demonstrated a polypeptide pattern identical with that of serum C1q on SDS/polyacrylamide-gel electrophoresis. Under non-reducing conditions two protein bands were detected migrating with the same Rf values as the serum C1q A-B and C-C dimers. On reduction three bands were evident, which migrated identically with the A, B and C chains of serum C1q. The amount of radioactivity in these bands increased with time in culture, consistent with the e.l.i.s.a. and haemolytic C1q assays. These bands were reactive with monospecific anti-C1q antibody after transfer to nitrocellulose.

摘要

采用一种能够定量低至2 ng/ml的C1q浓度的酶联免疫吸附测定法(ELISA)和一种灵敏的溶血测定法,来研究与人血清C1q发生交叉反应的物质的出现情况以及人单核细胞培养基中的C1q溶血活性。在培养10 - 14天后在培养基中检测到这种物质,并且在培养至第28天(此时培养终止)时持续分泌。用[3H]脯氨酸或[35S]甲硫氨酸进行代谢标记的细胞培养基中,经琼脂糖-抗C1q抗体特异性免疫吸附的物质,在SDS/聚丙烯酰胺凝胶电泳上显示出与血清C1q相同的多肽图谱。在非还原条件下,检测到两条蛋白带,其迁移率与血清C1q A - B和C - C二聚体相同。还原后出现三条明显的带,其迁移情况与血清C1q的A、B和C链相同。这些条带中的放射性量随培养时间增加,这与ELISA和溶血C1q测定结果一致。转移至硝酸纤维素膜后,这些条带与单特异性抗C1q抗体发生反应。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/127f/1153046/99e1bbd737f9/biochemj00287-0143-a.jpg

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