中华医学遗传学杂志
中華醫學遺傳學雜誌
중화의학유전학잡지
CHINESE JOURNAL OF MEDICAL GENETICS
2014年
4期
487-490
,共4页
许先国%刘瑛%应燕玲%洪小珍%马开荣%蓝小飞%陈舒%何吉%朱发明
許先國%劉瑛%應燕玲%洪小珍%馬開榮%藍小飛%陳舒%何吉%硃髮明
허선국%류영%응연령%홍소진%마개영%람소비%진서%하길%주발명
血型%基因表达%细胞培养%红细胞
血型%基因錶達%細胞培養%紅細胞
혈형%기인표체%세포배양%홍세포
Blood group%Gene expression%Cell culture%Erythrocyte
目的 通过外周血非动员干细胞液培养获得红系有核细胞,以分析红系特异性表达的血型基因.方法 外周血经离心分离和免疫磁珠分选获得CD34+造血干细胞,体外液体定向培养生成红系有核细胞.分别取不同培养期的细胞进行免疫荧光和染色分析,并取培养+12 d的细胞进行Rh和ABO血型基因RNA转录分析.结果 从约50 mL外周血中分离到CD34+细胞(3.19±0.13)×104个(总回收率为67.3%±2.7%).经红系定向培养,大约+9d时细胞数爆增至平台期(7.57±0.78)×106个,扩增约237.1±15.5倍.在培养过程中,标志细胞干性的CD34抗原逐渐下降,红系特异性标志CD235a和CD240D逐渐上升.培养+12 d细胞提取的RNA,均能扩增出RHD/CE和ABO基因,DNA序列分析表明其基因型符合血清学表型.结论 建立了一种源于外周血非动员干细胞体外培养分析红系血型基因表达情况的方法,该技术可用于各种红系特异性表达基因的研究.
目的 通過外週血非動員榦細胞液培養穫得紅繫有覈細胞,以分析紅繫特異性錶達的血型基因.方法 外週血經離心分離和免疫磁珠分選穫得CD34+造血榦細胞,體外液體定嚮培養生成紅繫有覈細胞.分彆取不同培養期的細胞進行免疫熒光和染色分析,併取培養+12 d的細胞進行Rh和ABO血型基因RNA轉錄分析.結果 從約50 mL外週血中分離到CD34+細胞(3.19±0.13)×104箇(總迴收率為67.3%±2.7%).經紅繫定嚮培養,大約+9d時細胞數爆增至平檯期(7.57±0.78)×106箇,擴增約237.1±15.5倍.在培養過程中,標誌細胞榦性的CD34抗原逐漸下降,紅繫特異性標誌CD235a和CD240D逐漸上升.培養+12 d細胞提取的RNA,均能擴增齣RHD/CE和ABO基因,DNA序列分析錶明其基因型符閤血清學錶型.結論 建立瞭一種源于外週血非動員榦細胞體外培養分析紅繫血型基因錶達情況的方法,該技術可用于各種紅繫特異性錶達基因的研究.
목적 통과외주혈비동원간세포액배양획득홍계유핵세포,이분석홍계특이성표체적혈형기인.방법 외주혈경리심분리화면역자주분선획득CD34+조혈간세포,체외액체정향배양생성홍계유핵세포.분별취불동배양기적세포진행면역형광화염색분석,병취배양+12 d적세포진행Rh화ABO혈형기인RNA전록분석.결과 종약50 mL외주혈중분리도CD34+세포(3.19±0.13)×104개(총회수솔위67.3%±2.7%).경홍계정향배양,대약+9d시세포수폭증지평태기(7.57±0.78)×106개,확증약237.1±15.5배.재배양과정중,표지세포간성적CD34항원축점하강,홍계특이성표지CD235a화CD240D축점상승.배양+12 d세포제취적RNA,균능확증출RHD/CE화ABO기인,DNA서렬분석표명기기인형부합혈청학표형.결론 건립료일충원우외주혈비동원간세포체외배양분석홍계혈형기인표체정황적방법,해기술가용우각충홍계특이성표체기인적연구.
Objective To analyze specific expression of blood group genes using nucleated erythroid cells cultured from un-mobilized peripheral stem cells in vitro.Methods Hematopoietic stem cells(HSC) bearing the CD34 antigen were isolated from peripheral blood by centrifugation and magnetic beads sorting,followed by suspension culture in vitro.Cells were collected from medium on various stages and analyzed by immunofluorescence.The RNA transcription of RH and ABO blood group genes was analyzed using culture cells on day 12.Results A total of(3.19 ± 0.13) × 104 CD34 + cells were isolated from about 50 mL peripheral blood with a recovery rate of 67.3% ± 2.7%.The cells amount in erythroid-lineage culture system on day 9 reached a plateau of a 237.1±15.5-fold amplification of the initial cell input.The stem cell-specific CD34 antigen was dropped off,while the erythroid-specific CD235a and CD240D antigens were increased in culture period.RHD/CE and ABO genes can be amplified using RNA extracted from culture cells on day 12,and genotypes of Rh and ABO systems by DNA sequencing were consistent with their serologic phenotypes.Conclusion A method was established to analyze the gene expression of erythroid blood group derived from un-mobilized peripheral stem cells cultured in vitro.It can be used to study the expression of various erythroid-specific genes.
