设计 Ad5F35 载体以协调候选人类造血干细胞中的双重基因表达。

Design of Ad5F35 vectors for coordinated dual gene expression in candidate human hematopoietic stem cells.

机构信息

The Rausing Laboratory, Lund University, SE-221 84 Lund, Sweden.

出版信息

Exp Hematol. 2010 Jun;38(6):446-52. doi: 10.1016/j.exphem.2010.03.007. Epub 2010 Mar 18.

DOI:10.1016/j.exphem.2010.03.007

PMID:20303383

Abstract

OBJECTIVE

Adenoviral vector-mediated gene expression is an attractive approach to manipulate or report gene expression in human hematopoietic stem cells (HSC) when transient gene expression is preferred. Previous studies have demonstrated that fiber-retargeted Ad5F35 vectors can mediate efficient gene transfer into human HSCs. In this study, we investigated the potential of bi-directional promoter-controlled Ad5F35 vector for coordinated dual gene expression in candidate HSCs.

MATERIALS AND METHODS

We have engineered Ad5F35-DeltaLNGFR-BiDp encoding kinase domain deleted low-affinity NGF receptor (DeltaLNGFR) and green fluorescent protein (GFP) expression cassette controlled by a synthetic bi-directional promoter, which is composed of human phosphoglycerate kinase promoter and minimal core promoter from human cytomegalovirus. The expression pattern of DeltaLNGFR and GFP following Ad5F35-DeltaLNGFR-BiDp gene transfer in various cell types, including candidate HSCs, was compared to Ad5F35-DeltaLNGFR-IRES vector encoding phosphoglycerate kinase promoter-controlled bicistronic expression cassette for DeltaLNGFR and GFP.

RESULTS

Using Ad5F35-DeltaLNGFR-BiDp, we demonstrated a coordinated, high-level dual gene expression in leukemic cells and cord blood CD34(+) cells. However, the ability of Ad5F35-DeltaLNGFR-BiDp-GFP for coordinated dual gene expression varied significantly between repopulating progenitor cells. In nonobese diabetic severe combined immune deficient mice bone marrow transplantation assay, sorted CD34(+)/DeltaLNGFR(+)/GFP(+) cells following infection with Ad5F35-DeltaLNGFR-BiDp showed predominantly myeloid lineage reconstitution with limited lymphoid lineage differentiation capacity, whereas the CD34(+)/DeltaLNGFR(+)/GFP(-) cells exhibited both myeloid and lymphoid reconstitution.

CONCLUSIONS

This study indicates that bi-directional promoter-controlled Ad5F35 vector, such as Ad5F35-DeltaLNGFR-BiDp, can be particularly useful for manipulation of myeloid progenitor cells and potentially in myeloid lineage leukemic cells as well.

摘要

目的

当需要瞬时基因表达时，腺病毒载体介导的基因表达是一种在人造血干细胞（HSC）中操纵或报告基因表达的有吸引力的方法。先前的研究表明，纤维靶向的 Ad5F35 载体可以有效地将基因转移到人 HSC 中。在这项研究中，我们研究了双启动子控制的 Ad5F35 载体在候选 HSC 中协调双重基因表达的潜力。

材料和方法

我们设计了 Ad5F35-DeltaLNGFR-BiDp，该载体编码已删除激酶结构域的低亲和力神经生长因子受体（DeltaLNGFR）和绿色荧光蛋白（GFP）表达盒，由人磷酸甘油酸激酶启动子和来自人巨细胞病毒的最小核心启动子组成的合成双向启动子控制。比较了 Ad5F35-DeltaLNGFR-BiDp 基因转移后候选 HSC 等各种细胞类型中 DeltaLNGFR 和 GFP 的表达模式与 Ad5F35-DeltaLNGFR-IRES 载体（编码磷酸甘油酸激酶启动子控制的双顺反子表达盒用于 DeltaLNGFR 和 GFP）。

结果

使用 Ad5F35-DeltaLNGFR-BiDp，我们在白血病细胞和脐血 CD34+细胞中证明了协调的高水平双重基因表达。然而，Ad5F35-DeltaLNGFR-BiDp-GFP 协调双重基因表达的能力在重编程祖细胞之间差异很大。在非肥胖型糖尿病严重联合免疫缺陷小鼠骨髓移植实验中，用 Ad5F35-DeltaLNGFR-BiDp 感染后分选的 CD34+/DeltaLNGFR+/GFP+细胞主要表现出骨髓谱系重建，具有有限的淋巴谱系分化能力，而 CD34+/DeltaLNGFR+/GFP-细胞则表现出骨髓和淋巴谱系重建。