首页> 外文期刊>Journal of hematotherapy and stem cell research >Comparison of progenitor cell collection on day 4 or day 5 after steady-state stimulation with G-CSF alone in breast cancer patients: influence on CD34+ cell yield, subpopulation, and breast cancer cell contamination.
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Comparison of progenitor cell collection on day 4 or day 5 after steady-state stimulation with G-CSF alone in breast cancer patients: influence on CD34+ cell yield, subpopulation, and breast cancer cell contamination.

机译:乳腺癌患者仅接受G-CSF稳态刺激后第4天或第5天收集祖细胞的比较:对CD34 +细胞产量,亚群和乳腺癌细胞污染的影响。

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To determine the influence of apheresis timing on CD34+ cell yield, subpopulation, and breast cancer cell contamination, 48 women with breast cancer were stimulated from steady-state hematopoiesis in a prospective but nonrandomized study with 2 x 5 microg/kg G-CSF s.c. alone, and apheresis was started either on day 4 (n = 24) or day 5 (n = 24). Forty-eight women with breast cancer (stage II/III, n = 30; stage IV; n = 12; inflammatory, n = 6) and a median age of 44 years were well balanced between the two groups. In group I, aphersis was started on day 4 and additionally performed on day 5 after G-CSF stimulation, and in group II, apheresis was started on day 5. CD34+ cell count and CD34+ cell subpopulation were determined according to international criteria. Breast cancer cell contamination was detected by immunocytology. The median CD34+ cell harvest on day 4 was 3.3 x 10(6)/kg body weight (range 0.5-12.8) and 6 x 10(6)/kg BW (range 0.3-30) for patients starting on day 5 (p = 0.01). Those patients starting on day 4 achieved a median CD34+ cell count of 4 x 10(6)/kg (range 0.7-13) on day 5 (NS). Twenty-one percent of group I and 71% of group II achieved >5 x 10(6)/kg BW CD34+ cells in the first apheresis, whereas <2.5 x 10(6)/kg BW CD34+ cells in the first apheresis were observed in 38% of group I and 16% of group II. No differences were observed between the CD34+ cell subpopulations, CD34+/CD38+ (10.5% versus 10.5%) and CD34+/Thyl+ (1.5% versus 1.8%). The CD34+ cell harvest from consecutive collecting on days 4 and 5 was nearly identical to the harvest starting on day 5 (6.4 versus 6 x 10(6)/kg). Collecting CD34+ progenitor cells after stimulation with G-CSF alone on day 5 results in a significantly higher cell yield than starting collecting on day 4. No differences in respect to breast cancer cell contamination and CD34+ cell subpopulation were observed.
机译:为了确定单采血液时机对CD34 +细胞产量,亚群和乳腺癌细胞污染的影响,在一项前瞻性但非随机的研究中,以2 x 5 microg / kg G-CSF s.c刺激了48名患有稳态造血功能的乳腺癌女性。单独进行,并在第4天(n = 24)或第5天(n = 24)开始采血。两组女性中有48位患有乳腺癌(II / III期,n = 30; IV期; n = 12;炎性,n = 6),中位年龄为44岁。第一组,在G-CSF刺激后第4天开始单采血液,另外在第5天进行单卵,第二组在第5天开始单采血液。根据国际标准确定CD34 +细胞计数和CD34 +细胞亚群。通过免疫细胞学检测乳腺癌细胞污染。从第5天开始,患者第4天的平均CD34 +细胞收获量为3.3 x 10(6)/ kg体重(范围0.5-12.8)和6 x 10(6)/ kg BW(范围0.3-30)(p = 0.01)。从第4天开始的那些患者在第5天(NS)获得的CD34 +细胞计数中位数为4 x 10(6)/ kg(范围0.7-13)。 I组的21%和II组的71%在第一次采血中获得了> 5 x 10(6)/ kg BW CD34 +细胞,而在第一次采血中观察到了<2.5 x 10(6)/ kg BW CD34 +细胞在第一组的38%和第二组的16%中。在CD34 +细胞亚群,CD34 + / CD38 +(10.5%对10.5%)和CD34 + / Thyl +(1.5%对1.8%)之间未观察到差异。在第4天和第5天连续收集的CD34 +细胞收获与从第5天开始的收获几乎相同(6.4对6 x 10(6)/ kg)。在第5天单独用G-CSF刺激后,收集CD34 +祖细胞比第4天开始收集时,细胞产量显着提高。未观察到乳腺癌细胞污染和CD34 +细胞亚群方面的差异。

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