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Comparison of three retroviral vector systems for transduction of nonobese diabetic/severe combined immunodeficiency mice repopulating human CD34+ cord blood cells.三种逆转录病毒载体系统转导重建造血人CD34+脐血细胞的非肥胖糖尿病/严重联合免疫缺陷小鼠的比较。
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Transduction of umbilical cord blood CD34+ NOD/SCID-repopulating cells by simian foamy virus type 1 (SFV-1) vector.1型猿猴泡沫病毒(SFV-1)载体对脐带血CD34+ NOD/SCID重建造血细胞的转导
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Transduction of human NOD/SCID-repopulating cells with both lymphoid and myeloid potential by foamy virus vectors.泡沫病毒载体转导具有淋巴样和髓样潜能的人NOD/SCID重建造血干细胞
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与致瘤病毒和慢病毒载体相比,泡沫病毒载体转导的细胞周期要求。

Cell cycle requirements for transduction by foamy virus vectors compared to those of oncovirus and lentivirus vectors.

作者信息

Trobridge Grant, Russell David W

机构信息

Department of Medicine, Division of Hematology, University of Washington, Seattle, Washington 98195, USA.

出版信息

J Virol. 2004 Mar;78(5):2327-35. doi: 10.1128/jvi.78.5.2327-2335.2004.

DOI:10.1128/jvi.78.5.2327-2335.2004
PMID:14963129
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC369213/
Abstract

Retroviral vectors based on foamy viruses (FV) are efficient gene delivery vehicles for therapeutic and research applications. While previous studies have shown that FV vectors transduce quiescent cell cultures more efficiently than oncoviral vectors, their specific cell cycle requirements have not been determined. Here we compare the transduction frequencies of FV vectors with those of onco- and lentiviral vectors in nondividing and dividing normal human fibroblasts by several methods. FV vectors transduced serum-deprived fibroblast cultures more efficiently than oncoretroviral vectors and at rates comparable to those of lentiviral vectors. However, in these cultures FV vectors only transduced a subpopulation of proliferating cells, as determined by bromodeoxyuridine staining for DNA synthesis. In contrast to lentiviral vectors, FV vectors were unable to transduce human fibroblasts arrested by aphidicolin (G(1)/S phase) or gamma-irradiation (G(2) phase), and a partial cell cycle that included mitosis but not DNA synthesis was required. We could not determine if mitosis facilitated nuclear entry of FV vectors, since cell-free vector preparations contained long terminal repeat circles, precluding their use as nuclear markers. In contrast to oncoviral vectors, both FV and lentiviral vectors efficiently transduced G(0) fibroblasts that were later stimulated to divide. In the case of FV vectors, this was due to the persistence of a stable transduction intermediate in quiescent cells. Our findings support the use of FV vectors as a safe and effective alternative to lentiviral vectors for ex vivo transduction of stem cells that are quiescent during culture but divide following transplantation.

摘要

基于泡沫病毒(FV)的逆转录病毒载体是用于治疗和研究应用的高效基因递送工具。虽然先前的研究表明,FV载体比致瘤病毒载体更有效地转导静止细胞培养物,但其特定的细胞周期要求尚未确定。在这里,我们通过几种方法比较了FV载体与致瘤病毒载体和慢病毒载体在未分裂和分裂的正常人成纤维细胞中的转导频率。FV载体比致瘤逆转录病毒载体更有效地转导血清饥饿的成纤维细胞培养物,其转导速率与慢病毒载体相当。然而,在这些培养物中,通过溴脱氧尿苷染色检测DNA合成发现,FV载体仅转导增殖细胞的一个亚群。与慢病毒载体不同,FV载体无法转导被阿非科林(G1/S期)或γ射线照射(G2期)阻滞的人成纤维细胞,并且需要一个包括有丝分裂但不包括DNA合成的部分细胞周期。由于无细胞载体制剂中含有长末端重复序列环,无法将其用作核标记,因此我们无法确定有丝分裂是否促进了FV载体进入细胞核。与致瘤病毒载体不同,FV和慢病毒载体都能有效地转导G0期成纤维细胞,这些细胞随后被刺激分裂。就FV载体而言,这是由于在静止细胞中存在稳定的转导中间体。我们的研究结果支持将FV载体用作慢病毒载体的安全有效替代品,用于体外转导在培养过程中静止但移植后分裂的干细胞。