Ponnazhagan S, Mukherjee P, Wang X S, Qing K, Kube D M, Mah C, Kurpad C, Yoder M C, Srour E F, Srivastava A
Department of Microbiology and Immunology, Walther Oncology Center, Indiana University School of Medicine, Indianapolis 46202, USA.
J Virol. 1997 Nov;71(11):8262-7. doi: 10.1128/JVI.71.11.8262-8267.1997.
Although the adeno-associated virus type 2 (AAV) is known to possess a broad host range that transcends the species barrier, we suggested in an earlier study that AAV infection of human cells is receptor mediated (S. Ponnazhagan et al., J. Gen. Virol. 77:1111-1122, 1996). In the present studies, we investigated the ability of AAV to infect primary human hematopoietic progenitor cells capable of multilineage differentiation. Bone marrow-derived CD34+ cells from 12 hematologically normal volunteer donors were infected with a recombinant AAV containing the beta-galactosidase gene under the control of the cytomegalovirus immediate-early promoter (vCMVp-lacZ). Whereas 15 to 80% of the cells from approximately 50% of the donors showed various levels of lacZ gene expression, the expression was undetectable in cells from the remaining donors. However, if cells from both sets of donors were stimulated with various combinations of cytokines to induce differentiation into myeloid and lymphoid lineages following AAV infection, then the level of expression of the transduced gene increased up to 20-fold over a period of 14 days. The results of virus-binding assays suggested that the observed difference between the two groups was due to the differential susceptibility of CD34+ cells to AAV infection rather than to differences in transcription and translation of the transduced gene. To corroborate these results, CD34+ cells from the two donor groups, KB (human nasopharyngeal carcinoma) cells, and M07e (human megakaryocytic leukemia) cells were infected with vCMVp-lacZ. KB cells served as a positive control for AAV infection, and M07e cells served as a negative control. Whereas abundant hybridization to the single-stranded viral DNA on Southern blots was detected in KB and CD34+ cells that were positive for lacZ gene expression, little activity was detected in M07e and CD34+ cells that did not show expression of the lacZ gene. These results suggest that the levels of expression of the putative cellular receptor for AAV vary widely in CD34+ cells from different donors. These studies have implications for the potential use of AAV vectors in human gene therapy involving primary human primitive hematopoietic stem and progenitor cells.
尽管已知2型腺相关病毒(AAV)具有跨越物种屏障的广泛宿主范围,但我们在早期研究中提出,AAV对人类细胞的感染是受体介导的(S. Ponnazhagan等人,《普通病毒学杂志》77:1111 - 1122,1996)。在本研究中,我们调查了AAV感染能够进行多谱系分化的原代人类造血祖细胞的能力。来自12名血液学正常志愿者供体的骨髓来源的CD34 +细胞,用一种重组AAV感染,该重组AAV含有在巨细胞病毒立即早期启动子(vCMVp - lacZ)控制下的β - 半乳糖苷酶基因。大约50%的供体中,15%至80%的细胞显示出不同水平的lacZ基因表达,而其余供体的细胞中未检测到该表达。然而,如果两组供体的细胞在AAV感染后用各种细胞因子组合刺激以诱导分化为髓系和淋巴系谱系,那么在14天内转导基因的表达水平增加高达20倍。病毒结合试验结果表明,两组之间观察到的差异是由于CD34 +细胞对AAV感染的敏感性不同,而不是由于转导基因转录和翻译的差异。为了证实这些结果,将来自两组供体的CD34 +细胞、KB(人鼻咽癌)细胞和M07e(人巨核细胞白血病)细胞用vCMVp - lacZ感染。KB细胞用作AAV感染的阳性对照,M07e细胞用作阴性对照。在Southern印迹上,在lacZ基因表达阳性的KB和CD34 +细胞中检测到与单链病毒DNA的大量杂交,而在未显示lacZ基因表达的M07e和CD34 +细胞中几乎检测不到活性。这些结果表明,不同供体的CD34 +细胞中AAV假定细胞受体的表达水平差异很大。这些研究对于AAV载体在涉及原代人类原始造血干细胞和祖细胞的人类基因治疗中的潜在应用具有启示意义。
