一种用于流式细胞术检测B细胞慢性淋巴细胞白血病中ZAP-70的封闭抗体方法的应用。

Shenkin Mark, Maiese Russell

AmeriPath, Inc, Orlando, FL and Shelton, CT, USA.

Cytometry B Clin Cytom. 2006 Jul 15;70(4):251-8. doi: 10.1002/cyto.b.20125.

BACKGROUND

In this study we developed a method to measure the amount of ZAP-70 [zeta accessory protein] in B-CLL cells without relying on the ZAP-70 expression of patient B or T cells to normalize fluorescence intensity.

METHODS

B-CLL cells were fixed with formaldehyde before surface staining with gating antibodies CD19PC5 and CD5FITC. The cells were permeabilized with saponin, and the ZAP-70 antigen was blocked in one tube with unlabeled antibody to ZAP-70 [clone 1E7.2]. Zap-70-PE was then added to this tube. ZAP-70-PE was added to a second tube without unlabeled antibody to ZAP-70. The mean fluorescence intensity of the ZAP-70 in the tube without unlabeled antibody divided by the mean fluorescence intensity of the ZAP-70 in the tube with unlabeled antibody equals the RATIO of total fluorescence to non-specific ZAP-70 fluorescence in the B-CLL cells. In a second method of analysis, a region is created in the histogram showing ZAP-70 fluorescence intensity in the tube with unlabeled antibody to ZAP-70. This region is set to 0.9% positive cells. This same region is then used to measure the % positive [%POS] ZAP-70 cells in the tube without unlabeled antibody to ZAP-70. The brighter the ZAP-70 fluorescence above the non-specific background, the higher the %POS.

RESULTS

Due to the varying amount of non-specific staining between patient B-CLL cells and other cells, the blocking antibody method yielded a more quantitative and reproducible measure of ZAP-70 in B-CLL cells than other methods, which use the ratio of B-CLL fluorescence to normal B or T-cell fluorescence. Using this improved method, ZAP-70 was determined to be negative if the RATIO was less than 2:1 and positive if the RATIO was greater than 2:1. ZAP-70 was determined to be negative if the %POS was less than 5% and positive if the %POS was greater than 5%, a cut-off value lower than previous values published, due to exclusion of non-specific staining. Both cut-offs were based upon patient specimen distribution profiling.

CONCLUSIONS

Use of a blocking antibody resulted in a robust, reproducible clinical B-CLL assay that is not influenced by the need to measure the amount of ZAP-70 in other cells. ZAP-70 results segre gate patients into indolent and aggressive groups suggested by published clinical outcomes.

背景

在本研究中，我们开发了一种方法来测量B细胞慢性淋巴细胞白血病（B-CLL）细胞中ZAP-70（ζ辅助蛋白）的含量，而无需依赖患者B细胞或T细胞的ZAP-70表达来标准化荧光强度。

方法

在用门控抗体CD19PC5和CD5FITC进行表面染色之前，用甲醛固定B-CLL细胞。用皂苷使细胞通透，并用未标记的ZAP-70抗体（克隆1E7.2）在一管中封闭ZAP-70抗原。然后将ZAP-70-PE添加到该管中。将ZAP-70-PE添加到第二管中，该管中没有未标记的ZAP-70抗体。未加未标记抗体管中ZAP-70的平均荧光强度除以加了未标记抗体管中ZAP-70的平均荧光强度，等于B-CLL细胞中总荧光与非特异性ZAP-70荧光的比值。在第二种分析方法中，在直方图中创建一个区域，该区域显示加了未标记ZAP-70抗体管中的ZAP-70荧光强度。该区域设定为0.9%的阳性细胞。然后使用相同的区域来测量未加未标记ZAP-70抗体管中ZAP-70阳性细胞的百分比（%POS）。ZAP-70荧光在非特异性背景之上越亮，%POS越高。

结果

由于患者B-CLL细胞与其他细胞之间非特异性染色量的变化，与其他使用B-CLL荧光与正常B细胞或T细胞荧光比值的方法相比，封闭抗体法对B-CLL细胞中ZAP-70的测量更具定量性和可重复性。使用这种改进的方法，如果比值小于2:1，则ZAP-70被判定为阴性；如果比值大于2:1，则ZAP-70被判定为阳性。如果%POS小于5%，则ZAP-70被判定为阴性；如果%POS大于5%，则ZAP-70被判定为阳性，由于排除了非特异性染色，该临界值低于先前发表的值。这两个临界值均基于患者标本分布分析。