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皮内注射单核细胞趋化蛋白-1可诱导大鼠皮肤中血液单核细胞的迁出和分化。

Intradermal injection of monocyte chemoattractant protein-1 induces emigration and differentiation of blood monocytes in rat skin.

作者信息

Yamashiro S, Takeya M, Kuratsu J, Ushio Y, Takahashi K, Yoshimura T

机构信息

Second Department of Pathology, Kumamoto University School of Medicine, Japan.

出版信息

Int Arch Allergy Immunol. 1998 Jan;115(1):15-23. doi: 10.1159/000023825.

DOI:10.1159/000023825
PMID:9430491
Abstract

BACKGROUND

Monocyte chemoattractant protein-1 (MCP-1) is a potent chemoattractant for blood monocytes in vitro. Recent studies in MCP-1-transgenic mice revealed that the local production of MCP-1 caused monocyte infiltration. However, the kinetics of monocyte infiltration after the production of MCP-1 or the amount of MCP-1 necessary for monocyte recruitment are not known.

METHODS

We purified recombinant rat MCP-1 expressed in COS-7 cells, and injected it into rat skin. The infiltrating cells were examined by immunohistochemistry and ultrastructural peroxidase cytochemistry.

RESULTS

Rat recombinant MCP-1 had a molecular mass of approximately 30 kD and exhibited the peak monocyte chemotactic activity at 10(-9) M. One microgram of MCP-1 caused intra- and extravascular accumulation of mononuclear cells 3 h after injection. The cells were ED1+, indicating they were blood monocytes. The infiltration of mononuclear cells peaked at 12-24 h, and most of them were TRPM-3+ and ED3+, characteristic to exudate macrophages. None of the cells expressed ED2 or Ki-M2R antigens, markers for resident macrophages, until 3 days after injection. There was no uptake of [3H]thymidine by the infiltrating cells. Ultrastructural peroxidase cytochemistry confirmed that the infiltrating cells were monocytes and exudate macrophages. The number of OX8+ lymphocytes also peaked at 12 h, consisting of approximately 9% of the total infiltrating cells.

CONCLUSION

These results indicate that MCP-1 attracts blood monocytes as early as 3 h and the infiltrating monocytes differentiate into exudate macrophages in loco. However, this effect was transient and the infiltration of monocytes did not result in tissue damage.

摘要

背景

单核细胞趋化蛋白-1(MCP-1)在体外是一种对血液单核细胞有效的趋化因子。最近对MCP-1转基因小鼠的研究表明,MCP-1的局部产生会导致单核细胞浸润。然而,MCP-1产生后单核细胞浸润的动力学或单核细胞募集所需的MCP-1量尚不清楚。

方法

我们纯化了在COS-7细胞中表达的重组大鼠MCP-1,并将其注射到大鼠皮肤中。通过免疫组织化学和超微结构过氧化物酶细胞化学检查浸润细胞。

结果

大鼠重组MCP-1的分子量约为30 kD,在10^(-9) M时表现出峰值单核细胞趋化活性。注射1微克MCP-1后3小时,单核细胞在血管内和血管外积聚。这些细胞为ED1+,表明它们是血液单核细胞。单核细胞浸润在12 - 24小时达到峰值,其中大多数为TRPM-3+和ED3+,这是渗出性巨噬细胞的特征。直到注射后3天,没有细胞表达ED2或Ki-M2R抗原(驻留巨噬细胞的标志物)。浸润细胞没有摄取[3H]胸腺嘧啶核苷。超微结构过氧化物酶细胞化学证实浸润细胞是单核细胞和渗出性巨噬细胞。OX8+淋巴细胞的数量也在12小时达到峰值,约占总浸润细胞的9%。

结论

这些结果表明,MCP-1早在3小时就吸引血液单核细胞,浸润的单核细胞在局部分化为渗出性巨噬细胞。然而,这种作用是短暂的,单核细胞的浸润并未导致组织损伤。

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