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肺间质巨噬细胞:与肺泡巨噬细胞和血液单核细胞的分离及流式细胞术比较

Pulmonary interstitial macrophages: isolation and flow cytometric comparisons with alveolar macrophages and blood monocytes.

作者信息

Dethloff L A, Lehnert B E

机构信息

Toxicology Group, Los Alamos National Laboratory, NM 87545.

出版信息

J Leukoc Biol. 1988 Jan;43(1):80-90. doi: 10.1002/jlb.43.1.80.

Abstract

Pulmonary interstitial macrophages (IM) were isolated from rat lungs by an Fc gamma receptor-based affinity technique coupled with multiparameter flow cytometry. Single cell suspensions obtained by collagenase digestion of extensively perfused and lavaged lungs were applied to carpets of opsonized sheep red blood cells (SRBC-IgG) bound to plastic tissue culture flasks. At 0-4 degrees C, optimal binding of lung cells occurred within 60 min at plating densities of 1-2 X 10(6) lung cells/cm2 when the SRBC substrate was opsonized with 10 micrograms/ml anti-SRBC IgG. Nonadherent cells were removed by gently rinsing the plates and adherent cells were recovered by lysing the SRBC-IgG substrata. By light microscopy, the mixture of adherent cells was comprised of mononuclear cells (approximately 54%), many of which appeared to be macrophages, lymphocytes (approximately 20%), polymorphonuclear leukocytes (approximately 15%), plasma cells (approximately 8%), eosinophils (approximately 2%), and mast cells (approximately 0.5%). The cells which adhered to the SRBC-IgG monolayers were further resolved into subpopulations by multiparameter flow cytometry and sorted according to their electro-optical characteristics. One subpopulation appeared morphologically to be macrophages, and greater than 90% of these cells readily phagocytized SRBC-IgG in vitro. Peroxidase staining of this population was minimal, indicating that these cells were not blood monocytes (BM). Using a method by which alveolar macrophages (AM) were prelabeled with SRBC-IgG in situ, we demonstrated that alveolar macrophages constituted only approximately 5% of the total adherent cell population. We concluded from these observations that the macrophage population harvested in this manner were neither BM nor AM, but, rather, were harvested from the lung's interstitial compartment. Flow cytometric analyses indicated that the IM exhibited electro-optical characteristics intermediate between those of BM and AM, which is consistent with the concept of the lung's interstitium as a maturation compartment for the BM prior to migration into the alveolar compartment. However, the IM more closely resembled the BM than the AM, indicating that if the IM is in fact a precursor to the AM population, substantial maturation or differentiation must occur subsequent to its migration into the alveolar compartment. This isolation technique will be useful for harvesting highly purified IM for in vitro investigations.

摘要

通过基于Fcγ受体的亲和技术结合多参数流式细胞术从大鼠肺中分离出肺间质巨噬细胞(IM)。通过对充分灌注和灌洗的肺进行胶原酶消化获得的单细胞悬液,应用于与塑料组织培养瓶结合的调理过的绵羊红细胞(SRBC-IgG)铺片上。在0-4℃下,当SRBC底物用10μg/ml抗SRBC IgG调理时,肺细胞在接种密度为1-2×10(6)个肺细胞/cm2的情况下,60分钟内发生最佳结合。通过轻轻冲洗平板去除非贴壁细胞,并通过裂解SRBC-IgG底物回收贴壁细胞。通过光学显微镜观察,贴壁细胞混合物由单核细胞(约54%)组成,其中许多似乎是巨噬细胞、淋巴细胞(约20%)、多形核白细胞(约15%)、浆细胞(约8%)、嗜酸性粒细胞(约2%)和肥大细胞(约0.5%)。通过多参数流式细胞术将粘附于SRBC-IgG单层的细胞进一步解析为亚群,并根据其电光特性进行分选。一个亚群在形态上似乎是巨噬细胞,其中超过90%的细胞在体外易于吞噬SRBC-IgG。该群体的过氧化物酶染色极少,表明这些细胞不是血液单核细胞(BM)。使用一种在原位用SRBC-IgG预标记肺泡巨噬细胞(AM)的方法,我们证明肺泡巨噬细胞仅占总贴壁细胞群体的约5%。我们从这些观察结果得出结论,以这种方式收获的巨噬细胞群体既不是BM也不是AM,而是从肺间质区室收获的。流式细胞术分析表明,IM表现出介于BM和AM之间的电光特性,这与肺间质作为BM迁移到肺泡区室之前的成熟区室的概念一致。然而,IM比AM更类似于BM,这表明如果IM实际上是AM群体的前体,则在其迁移到肺泡区室之后必须发生大量的成熟或分化。这种分离技术将有助于收获高度纯化的IM用于体外研究。

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