Reproducible scoring of CFU-GM and BFU-E grown in collagen-based semisolid medium after a short (3 h) training

被引:7
作者
Dobo, I
Bidet, JM
Acquart, S
Allegraud, A
Amiot, L
Boccaccio, C
Boiret, N
Domenech, J
Mossuz, P
Sensebe, L
Wunder, E
Zandecki, M
Hermouet, S
机构
[1] Etablissements Transfus Sanguine, Lab Cultures Cellulaires, Angers, France
[2] Etablissements Transfus Sanguine, Lab Cultures Cellulaires, St Etienne, France
[3] Ctr Hematol Paris La Pitie Salpetriere, Paris, France
[4] CHU Angers, Hematol Lab, Angers, France
[5] CHU Limoges, Hematol Lab, Limoges, France
[6] CHU Rennes, Hematol Lab, Rennes, France
[7] CHU Clermont Ferrand, Hematol Lab, Clermont Ferrand, France
[8] CHU Tours, Hematol Lab, Tours, France
[9] CHU Grenoble, Hematol Lab, Grenoble, France
[10] CHU Brest, Hematol Lab, Brest, France
[11] CHU Mulhouse, Hematol Lab, Mulhouse, France
[12] CHU Nantes, Hematol Lab, F-44035 Nantes 01, France
来源
JOURNAL OF HEMATOTHERAPY | 1999年 / 8卷 / 01期
关键词
D O I
10.1089/106161299320569
中图分类号
R5 [内科学];
学科分类号
1002 ; 100201 ;
摘要
Colony counting remains an important source of variation in colony-forming unit-granulocyte-macrophage (CFU-GM) assays performed in methylcellulose or agar. We studied the reliability of colony scoring of CFU-GM assays carried out with collagen, a matrix that allows gel collection on glass slides and in situ cellular morphology. Fourteen slides were exchanged among laboratories, and two rounds of colony (CFU-GM and burst-forming units-erythrocyte [BFU-E]) counting were performed by 11 (first counting), then 8 (second counting) different laboratories, the majority of which had no previous experience of collagen gel cultures and reading. Two-way analysis of variance (ANOVA) of the first round of colony counting showed significant differences among centers in CFU-GM counts (p = 0.023) but not in BFU-E counts (p = 0.163). Coefficients of variation for the 14 slides ranged from 22% to 50% (median 28%) for CFU-GM counts and from 12% to 74% (median 23%) for BFU-E counts. After a 3 h session of collective colony reading attended by members of 8 laboratories, a second round of colony counting was performed. This time, ANOVA showed no significant difference among centers for CFU-GM (p = 0.533) and BFU-E (p = 0.328) counts, and coefficients of variation were significantly improved, with medians of 17% for CFU-GM counts and 20% for BFU-E counts. In addition, when data from the second round of readings were analyzed without the 2 centers counting consistently low (center 8) or consistently high (center 5), variance among centers was further improved for both CFU-GM (p = 0.798) and BFU-E (p = 0.619). In summary, this study shows for the first time that reproducible BFU-E and CFU-GM scoring can be achieved using collagen-based semisolid medium (now commercially available) as long as adequate training in colony identification is provided.
引用
收藏
页码:45 / 51
页数:7
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