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人淋巴细胞上的膜免疫球蛋白:人扁桃体细胞表面IgD和IgM的周转率

Membrane Ig on human lymphocytes: rate of turnover of IgD and IgM on the surface of human tonsil cells.

作者信息

Ferrarini M, Corte G, Viale G, Durante M L, Bargellesi A

出版信息

Eur J Immunol. 1976 May;6(5):372-8. doi: 10.1002/eji.1830060513.

DOI:10.1002/eji.1830060513
PMID:991908
Abstract

The turnover of IgM and IgD molecules present on the membrane of human tonsil cells has been studied using immunofluorescence and peroxidase-catalyzed membrane radioiodination. With the first of the two techniques cells were treated with pronase to remove membrane immunoglobulin (mIg), placed in culture and stained at intervals to check the reappearance of membrane IgD and IgM on the cell membrane. These experiments showed that membrane IgD (in contrast to membrane IgM) are extremely susceptible to proteolysis. Furthermore, cells treated with a concentration of pronase found to be optimal to remove membrane IgM failed to re-express membrane IgD in vitro. The large majority of tonsil lymphocytes has both membrane IgM and IgD. Due to the different behavior of reappearance of the two membrane molecules after treatment with pronase, it was not possible to obtain the simultaneous re-expression of membrane IgM and IgD by the cells "stripped" with pronase. However, the two molecules were re-expressed in vitro by the cells treated with different pronase concentrations with a similar timing, i.e. 50% or more of the cells re-expressed membrane IgD and IgM after 8 h in culture. 131I-radioiodinated membrane IgD and IgM were also released from the cell surface with a similar timing, the half-life of permanence on the cell membrane being about 4 h for both molecules. These findings thus indicate that IgM and IgD molecules have a similar turnover and that a cell is capable of placing two different Ig molecules at a time on its surface.

摘要

利用免疫荧光和过氧化物酶催化的膜放射性碘化技术,对人扁桃体细胞膜上存在的IgM和IgD分子的周转情况进行了研究。采用这两种技术中的第一种,用链霉蛋白酶处理细胞以去除膜免疫球蛋白(mIg),将其置于培养中,并定期染色以检查细胞膜上膜IgD和IgM的重新出现情况。这些实验表明,膜IgD(与膜IgM相反)极易受到蛋白水解作用的影响。此外,用发现能最佳去除膜IgM的链霉蛋白酶浓度处理的细胞,在体外未能重新表达膜IgD。绝大多数扁桃体淋巴细胞同时具有膜IgM和膜IgD。由于用链霉蛋白酶处理后两种膜分子重新出现的行为不同,用链霉蛋白酶“剥离”的细胞不可能同时重新表达膜IgM和膜IgD。然而,用不同链霉蛋白酶浓度处理的细胞在体外以相似的时间重新表达了这两种分子,即培养8小时后,50%或更多的细胞重新表达了膜IgD和膜IgM。131I放射性碘化的膜IgD和膜IgM也以相似的时间从细胞表面释放,两种分子在细胞膜上的存留半衰期约为4小时。因此,这些发现表明IgM和IgD分子具有相似的周转情况,并且一个细胞能够同时在其表面放置两种不同的Ig分子。

相似文献

1
Membrane Ig on human lymphocytes: rate of turnover of IgD and IgM on the surface of human tonsil cells.人淋巴细胞上的膜免疫球蛋白:人扁桃体细胞表面IgD和IgM的周转率
Eur J Immunol. 1976 May;6(5):372-8. doi: 10.1002/eji.1830060513.
2
Membrane IgD and membrane IgM differ in capacity to transduce inhibitory signals within the same human B cell clonal populations.膜免疫球蛋白D(mIgD)和膜免疫球蛋白M(mIgM)在转导同一人类B细胞克隆群体内抑制性信号的能力上存在差异。
J Immunol. 1989 Sep 1;143(5):1565-74.
3
A study of immunoglobulin classes present on the membrane and in the cytoplasm of human tonsil plasma cells.对人扁桃体浆细胞膜上和细胞质中存在的免疫球蛋白类别的研究。
Eur J Immunol. 1976 Aug;6(8):562-5. doi: 10.1002/eji.1830060807.
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IgD expression on B cells is more efficient than IgM but both receptors are functionally equivalent in up-regulation CD80/CD86 co-stimulatory molecules.B细胞上IgD的表达比IgM更有效,但在上调CD80/CD86共刺激分子方面,这两种受体在功能上是等效的。
Eur J Immunol. 1995 Jul;25(7):1980-4. doi: 10.1002/eji.1830250727.
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In vitro studies on human IgD. I. Sources and characteristics of "externalized" IgD in tonsil lymphocyte cultures.人IgD的体外研究。I. 扁桃体淋巴细胞培养物中“外化”IgD的来源和特性。
Eur J Immunol. 1987 Apr;17(4):483-9. doi: 10.1002/eji.1830170408.
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Interaction of staphylococcal protein A with membrane components of IgM- and/or IgD-bearing lymphocytes from human tonsil.金黄色葡萄球菌蛋白A与人扁桃体中携带IgM和/或IgD的淋巴细胞膜成分的相互作用。
J Immunol. 1980 Apr;124(4):1620-6.
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Turnover of radioiodinated and of leucine-labeled immunoglobulin M in murine splenic lymphocytes.小鼠脾淋巴细胞中放射性碘标记和亮氨酸标记的免疫球蛋白M的周转率。
Eur J Immunol. 1975 Apr;5(4):234-40. doi: 10.1002/eji.1830050403.
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Cell surface immunoglobulin. XIX. Susceptibility of IgD and IgM on murine splenocytes to cleavage by papain.细胞表面免疫球蛋白。十九。小鼠脾细胞上IgD和IgM对木瓜蛋白酶裂解的敏感性。
J Immunol. 1976 Nov;117(5 Pt 1):1579-83.
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IgM and IgG but not cytokine secretion is restricted to the CD27+ B lymphocyte subset.IgM和IgG,但细胞因子分泌并不局限于CD27 + B淋巴细胞亚群。
J Immunol. 1992 Jun 15;148(12):3700-5.
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Membrane IgM and IgD molecules fail to transduce Ca2+ mobilizing signals when expressed on differentiated B lineage cells.当膜IgM和IgD分子在分化的B淋巴细胞系细胞上表达时,它们无法转导钙离子动员信号。
J Immunol. 1990 May 1;144(9):3272-80.

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Immunity. 2010 Mar 26;32(3):355-66. doi: 10.1016/j.immuni.2010.02.013. Epub 2010 Mar 11.
2
The normal counterpart of IgD myeloma cells in germinal center displays extensively mutated IgVH gene, Cmu-Cdelta switch, and lambda light chain expression.生发中心中IgD骨髓瘤细胞的正常对应物表现出广泛突变的IgVH基因、Cmu-Cdelta转换和λ轻链表达。
J Exp Med. 1998 Apr 20;187(8):1169-78. doi: 10.1084/jem.187.8.1169.
3
Simultaneous expression of mouse immunoglobulins M and D is determined by the same homolog of chromosome 12.
小鼠免疫球蛋白M和D的同时表达由12号染色体的同系物决定。
Proc Natl Acad Sci U S A. 1980 Nov;77(11):6793-6. doi: 10.1073/pnas.77.11.6793.
4
Study of proteolytic removal of Fab delta and Fe delta determinants of lymphocyte membrane IgD using a direct rosette assay.利用直接玫瑰花结试验对淋巴细胞膜IgD的Fabδ和Feδ决定簇进行蛋白水解去除的研究。
Immunology. 1981 Sep;44(1):89-95.