Introduction
To provide target values for the manufacturers’ survey of the Japanese Society for Laboratory Hematology (JSLH), accurate standard data from healthy volunteers were needed for the five‐part differential leukocyte count. To obtain such data, JSLH required an antibody panel that achieved high specificity (particularly for mononuclear cells) using simple gating procedures. We developed a flow cytometric method for determining the differential leukocyte count (JSLH‐Diff) and validated it by comparison with the flow cytometric differential leukocyte count of the International Council for Standardization in Haematology (ICSH‐Diff) and the manual differential count obtained by microscopy (Manual‐Diff).
Methods
First, the reference laboratory performed an imprecision study of JSLH‐Diff and ICSH‐Diff, as well as performing comparison among JSLH‐Diff, Manual‐Diff, and ICSH‐Diff. Then two reference laboratories and seven participating laboratories performed imprecision and accuracy studies of JSLH‐Diff, Manual‐Diff, and ICSH‐Diff. Simultaneously, six manufacturers’ laboratories provided their own representative values by using automated hematology analyzers.
Results
The precision of both JSLH‐Diff and ICSH‐Diff methods was adequate. Comparison by the reference laboratory showed that all correlation coefficients, slopes and intercepts obtained by the JSLH‐Diff, ICSH‐Diff, and Manual‐Diff methods conformed to the criteria. When the imprecision and accuracy of JSLH‐Diff were assessed at seven laboratories, the CV% for lymphocytes, neutrophils, monocytes, eosinophils, and basophils was 0.5~0.9%, 0.3~0.7%, 1.7~2.6%, 3.0~7.9%, and 3.8~10.4%, respectively. More than 99% of CD45 positive leukocytes were identified as normal leukocytes by JSLH‐Diff.
Conclusions
When JSLH‐Diff method were validated by comparison with Manual‐Diff and ICSH‐Diff, JSLH‐Diff showed good performance as a reference method.