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通过流式细胞术分析组胺及组胺类似物与淋巴细胞亚群的结合情况。

Binding of histamine and histamine analogs to lymphocyte subsets analyzed by flow cytometry.

作者信息

Muirhead K, Bender P, Hanna N, Poste G

出版信息

J Immunol. 1985 Dec;135(6):4120-8.

PMID:2415600
Abstract

The binding of histamine, 4-methylhistamine (a histamine type 2 receptor agonist), cimetidine (a histamine type 2 receptor antagonist), and telemethylhistamine (an inactive analog) to human peripheral blood mononuclear cell subsets was investigated by flow cytometry by using conjugates of these ligands coupled to fluorescein-labeled human serum albumin. Our results indicate that binding of fluorescent protein conjugates of histamine and its analogs does not selectively identify a lymphocyte subset(s) that mediates the immunomodulatory effects of histaminergic ligands. Conjugates with both low (2.5 to 2.8:1) and high (28 to 57:1) ligand to protein coupling ratios were used. No binding above background could be detected for the low mole ratio reagents. The high mole ratio reagents were bound by 95 to 99% of all lymphocytes when used at ligand concentrations of 50 microM or greater. At lower ligand concentrations, the number of lymphocytes exceeding a set fluorescence threshold was decreased, but fluorescence distributions remained unimodal at all concentrations used (1 to 500 microM). Monocytes also bound the high mole ratio reagents and gave rise to a second high-intensity peak in the fluorescence distribution unless they were excluded by other means. Levels of conjugate binding detected by flow cytometry did not parallel ligand potencies at classical histamine type 2 receptors; at equivalent ligand concentrations, approximately equal amounts of histamine or 4-methylhistamine conjugate were bound per lymphocyte, and only 30% less telemethylhistamine conjugate was bound. Competition with free ligands (10(2)- to 10(4)-fold excess histamine, 4-methylhistamine, cimetidine, or telemethylhistamine) did not significantly decrease the level of binding observed for the high mole ratio reagents at bound ligand concentrations of 1 to 25 microM. Dual staining with fluorescein-labeled conjugate and phycoerythrin-labeled monoclonal antibodies Leu-3ab (anti-helper T), Leu-2a (anti-suppressor T), Leu-M3 (anti-monocyte), or anti-HLA-DR (B cells and monocytes) was also carried out. The extent of conjugate binding to helper and suppressor cells was identical for each of the ligands used, but higher levels of conjugate binding were seen for monocytes and B cells than for T cells in every case. Our data do not exclude the possibility of enhanced conjugate binding to small numbers of activated (HLA-DR positive) T cells that might be involved in mediation of histamine effects.(ABSTRACT TRUNCATED AT 400 WORDS)

摘要

通过流式细胞术,利用与荧光素标记的人血清白蛋白偶联的这些配体的缀合物,研究了组胺、4-甲基组胺(一种组胺2型受体激动剂)、西咪替丁(一种组胺2型受体拮抗剂)和远甲基组胺(一种无活性类似物)与人外周血单个核细胞亚群的结合情况。我们的结果表明,组胺及其类似物的荧光蛋白缀合物的结合并不能选择性地识别介导组胺能配体免疫调节作用的淋巴细胞亚群。使用了低(2.5至2.8:1)和高(28至57:1)配体与蛋白偶联比的缀合物。对于低摩尔比试剂,未检测到高于背景的结合。当以50 microM或更高的配体浓度使用时,高摩尔比试剂与所有淋巴细胞的95%至99%结合。在较低的配体浓度下,超过设定荧光阈值的淋巴细胞数量减少,但在所有使用的浓度(1至500 microM)下,荧光分布仍保持单峰。单核细胞也结合高摩尔比试剂,并在荧光分布中产生第二个高强度峰,除非通过其他方法将其排除。通过流式细胞术检测到的缀合物结合水平与经典组胺2型受体处的配体效力不平行;在等效配体浓度下,每个淋巴细胞结合的组胺或4-甲基组胺缀合物量大致相等,而结合的远甲基组胺缀合物仅少30%。用游离配体(10²至10⁴倍过量的组胺、4-甲基组胺、西咪替丁或远甲基组胺)进行竞争,在1至25 microM的结合配体浓度下,并未显著降低高摩尔比试剂观察到的结合水平。还进行了用荧光素标记的缀合物和藻红蛋白标记的单克隆抗体Leu-3ab(抗辅助性T细胞)、Leu-2a(抗抑制性T细胞)、Leu-M3(抗单核细胞)或抗HLA-DR(B细胞和单核细胞)的双重染色。所用的每种配体与辅助性和抑制性细胞的缀合物结合程度相同,但在每种情况下,单核细胞和B细胞的缀合物结合水平均高于T细胞。我们的数据并不排除缀合物与可能参与介导组胺效应的少量活化(HLA-DR阳性)T细胞结合增强的可能性。(摘要截短于400字)

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Agents Actions. 1988 Jun;24(1-2):26-34. doi: 10.1007/BF01968076.