Malley A, Stewart C C, Stewart S J, Waldbeser L, Bradley L M, Shiigi S M
Oregon Regional Primate Research Center, Beaverton 97006.
J Leukoc Biol. 1988 Jun;43(6):557-65. doi: 10.1002/jlb.43.6.557.
Attempts to analyze bone marrow-derived macrophages (BMDM) by flow cytometry have been prohibited because of their high autofluorescence. Using an autofluorescence reduction method of Steinkamp and Stewart to reduce the autofluorescence of BMDM, we were able to examine several macrophage populations for their expression of I-A, I-J, and Mac-1 cell surface determinants. Bone marrow cells examined immediately after removal from the femur contain 50-60% Mac 1-positive cells (mainly granulocytes). During the next few days granulocytes and nonmacrophage precursor cells die, and the number of Mac 1-positive cells decrease. Once the bone marrow cells have been maintained in L cell conditioned medium (LCM) for 2 to 3 days, the number of cells expressing Mac 1 increases rapidly from 20% to 98% during the next 3 to 4 days. Bone marrow cells grown in LCM do not express I-J until these cells have been in culture 3 to 4 days, and the number of cells expressing I-J (up to 90% positive) parallels the increase in macrophages. Bone marrow cells maintained in LCM did not express detectable I-A during the 14 days these cells were examined. Two other macrophage populations often used in a variety of immunological studies were analyzed by flow cytometry. We found that the majority (up to 80%) of peritoneal cells expressed I-A, and only 20% of peritoneal cells had I-J cell surface determinants. On the other hand, peritoneal exudate cells collected 4 days after thioglycolate medium treatment were predominantly I-J positive (up to 70%), and only about 30% of these cells expressed I-A cell surface antigens. The binding of anti-I-J IgM antibody to BMDM was not to Fc receptors because pretreating these cells with up to 25 micrograms of an IgG2a myeloma protein did not block anti-I-J antibody binding. The addition of 25-200 micrograms of monoclonal anti-Fc receptor antibody was also ineffective in blocking the binding of a monoclonal anti-I-Jk antibody to BMDM. Pretreatment of BMDM with the IgM fraction of several control IgM antibody preparations did not block the specific binding of fluoresceinated anti-I-J IgM antibody. BMDM provide a pure population of macrophages that express a significant level of cell surface I-J antigens. Bone marrow cells grown in LCM are essentially devoid of other contaminating cells, and the increase in the number of I-J-positive cells parallels the increase in macrophages in these cultures.(ABSTRACT TRUNCATED AT 250 WORDS)
由于骨髓来源的巨噬细胞(BMDM)具有高自发荧光,通过流式细胞术分析它们的尝试一直受到限制。使用Steinkamp和Stewart的自发荧光降低方法来降低BMDM的自发荧光,我们能够检测几个巨噬细胞群体的I-A、I-J和Mac-1细胞表面决定簇的表达。从股骨中取出后立即检查的骨髓细胞含有50%-60%的Mac 1阳性细胞(主要是粒细胞)。在接下来的几天里,粒细胞和非巨噬细胞前体细胞死亡,Mac 1阳性细胞数量减少。一旦骨髓细胞在L细胞条件培养基(LCM)中培养2至3天,表达Mac 1的细胞数量在接下来的3至4天内从20%迅速增加到98%。在LCM中生长的骨髓细胞在培养3至4天之前不表达I-J,表达I-J的细胞数量(高达90%阳性)与巨噬细胞的增加平行。在检查的14天内,在LCM中培养的骨髓细胞未表达可检测到的I-A。通过流式细胞术分析了另外两个常用于各种免疫学研究的巨噬细胞群体。我们发现,大多数(高达80%)的腹腔细胞表达I-A,只有20%的腹腔细胞具有I-J细胞表面决定簇。另一方面,在硫代乙醇酸盐培养基处理4天后收集的腹腔渗出细胞主要为I-J阳性(高达70%),这些细胞中只有约30%表达I-A细胞表面抗原。抗I-J IgM抗体与BMDM的结合不是与Fc受体结合,因为用高达25微克的IgG2a骨髓瘤蛋白预处理这些细胞并不能阻断抗I-J抗体的结合。添加25-200微克的单克隆抗Fc受体抗体也不能有效阻断单克隆抗I-Jk抗体与BMDM的结合。用几种对照IgM抗体制剂的IgM部分预处理BMDM不能阻断荧光素化抗I-J IgM抗体的特异性结合。BMDM提供了一群表达显著水平细胞表面I-J抗原的纯巨噬细胞。在LCM中生长的骨髓细胞基本上没有其他污染细胞,I-J阳性细胞数量的增加与这些培养物中巨噬细胞的增加平行。(摘要截短于250字)
