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一种用于人类脐带血移植的小鼠模型:近期胎儿和新生儿外周血细胞可在亚致死剂量照射的成年受体中实现长期骨髓植入。

A murine model for human cord blood transplantation: near-term fetal and neonatal peripheral blood cells can achieve long-term bone marrow engraftment in sublethally irradiated adult recipients.

作者信息

Scaradavou A, Isola L, Rubinstein P, Galperin Y, Najfeld V, Berlin D, Gordon J, Weinberg R S

机构信息

Department of Pediatrics, Memorial Sloan-Kettering Cancer Center, New York, USA.

出版信息

Blood. 1997 Feb 1;89(3):1089-99.

PMID:9028342
Abstract

The purposes of the research reported here were first to explore a murine model for human placental and umbilical cord blood transplantation and second to evaluate the engraftment ability of ex vivo cultured hematopoietic cells. Murine near-term fetal and neonatal peripheral blood (FNPB) cells, genetically marked with the human multiple drug resistance transgene (MDR1) were used for syngeneic transplants into sublethally irradiated adult mice. Donor cells were transplanted either fresh and untreated, or after ex vivo culture in the presence of the hematopoietic growth factors recombinant murine stem cell factor, recombinant human interleukin-3 (rHu IL-3), and rHu IL-6, in a liquid culture system. To evaluate, count, and characterize FNPB progenitor cell-derived colonies, neonatal mouse mononuclear cells were cultured directly in methylcellulose with growth factors. To assess their ex vivo expansion ability, FNPB mononuclear cells were first cultured in liquid medium for 3 to 8 days and then transferred to semisolid assay plates. Evaluation of the cell counts after liquid culture showed a 1.4- to 11.6-fold increase, and the numbers of colonies observed in methylcellulose were similar to those produced by fresh FNPB cells. Donor-type engraftment was demonstrated by polymerase chain reaction (PCR) amplification of the human MDR1 transgene in the peripheral blood of all surviving animals (5 of 7 recipients of the fresh, and 3 of 8 recipients of the ex vivo-cultured cells) 2 to 4 months after transplantation. The proportion of donor leukocytes in the peripheral blood of the recipients (chimerism) was evaluated using fluorescence in situ hybridization (FISH) analysis 4 to 6 months after transplantation and ranged from 2% to 26%. In addition, bone marrow cultures were obtained from two recipient animals: one had received fresh-untreated cells and was evaluated 8 months after transplant, the other had received ex vivo cultured cells and was tested 14 months after grafting. The derived hematopoietic colonies were tested by PCR and the transgene was detected, conclusively proving long-term engraftment of donor cells. These results indicate that FNPB transplants can be successfully performed in sublethally irradiated mice with and without ex vivo culture. Long-term donor-type engraftment with sustained chimerism has been demonstrated. Thus, murine neonatal blood grafts can be used as an animal model for cord blood transplantation for gene therapy studies where complete myeloablation is not desirable and partial replacement of defective marrow may be sufficient. Furthermore, the possibility of numerically expanding hematopoietic progenitor cells contained in neonatal blood without affecting their engraftment ability could facilitate use of cord blood grafts in adult recipients.

摘要

本文报道的研究目的,一是探索用于人类胎盘和脐带血移植的小鼠模型,二是评估体外培养的造血细胞的植入能力。将携带人类多药耐药转基因(MDR1)的小鼠近足月胎儿及新生儿外周血(FNPB)细胞,用于同基因移植到经亚致死剂量照射的成年小鼠体内。供体细胞要么新鲜且未经处理直接移植,要么在液体培养系统中,于造血生长因子重组小鼠干细胞因子、重组人白细胞介素-3(rHu IL-3)和rHu IL-6存在的情况下进行体外培养后移植。为了评估、计数和鉴定FNPB祖细胞衍生的集落,将新生小鼠单核细胞直接与生长因子一起在甲基纤维素中培养。为了评估其体外扩增能力,先将FNPB单核细胞在液体培养基中培养3至8天,然后转移至半固体检测平板。液体培养后的细胞计数评估显示增加了1.4至11.6倍,在甲基纤维素中观察到的集落数量与新鲜FNPB细胞产生的集落数量相似。移植后2至4个月,通过聚合酶链反应(PCR)扩增所有存活动物(新鲜细胞移植的7只受体中有5只,体外培养细胞移植的8只受体中有3只)外周血中的人类MDR1转基因,证明了供体类型的植入。移植后4至6个月,使用荧光原位杂交(FISH)分析评估受体外周血中供体白细胞的比例(嵌合率),范围为2%至26%。此外,从两只受体动物获取了骨髓培养物:一只接受了新鲜未处理的细胞,在移植后8个月进行评估,另一只接受了体外培养的细胞,在移植后14个月进行检测。通过PCR检测所衍生的造血集落,并检测到转基因,最终证明了供体细胞的长期植入。这些结果表明,无论是否进行体外培养,FNPB移植均可在经亚致死剂量照射的小鼠中成功进行。已证明存在长期供体类型的植入及持续的嵌合现象。因此,小鼠新生儿血液移植可作为脐带血移植的动物模型,用于基因治疗研究,在这些研究中不需要完全清髓,部分替代有缺陷的骨髓可能就足够了。此外,在不影响其植入能力的情况下对新生儿血液中所含造血祖细胞进行数量扩增的可能性,可能会促进脐带血移植在成年受体中的应用。

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