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ATP 结合盒转运蛋白调节腔肠素和 D-荧光素生物发光成像。

ATP-binding cassette transporters modulate both coelenterazine- and D-luciferin-based bioluminescence imaging.

机构信息

Department of Neurology and Radiology, Memorial Sloan-Kettering Cancer Center, New York, NY 10065, USA.

出版信息

Mol Imaging. 2011 Jun;10(3):215-26.

Abstract

Bioluminescence imaging (BLI) of luciferase reporters provides a cost-effective and sensitive means to image biological processes. However, transport of luciferase substrates across the cell membrane does affect BLI readout intensity from intact living cells. To investigate the effect of ATP-binding cassette (ABC) transporters on BLI readout, we generated click beetle (cLuc), firefly (fLuc), Renilla (rLuc), and Gaussia (gLuc) luciferase HEK-293 reporter cells that overexpressed different ABC transporters (ABCB1, ABCC1, and ABCG2). In vitro studies showed a significant BLI intensity decrease in intact cells compared to cell lysates, when ABCG2 was overexpressed in HEK-293/cLuc, fLuc, and rLuc cells. Selective ABC transporter inhibitors were also applied. Inhibition of ABCG2 activity increased the BLI intensity more than two-fold in HEK-293/cLuc, fLuc, and rLuc cells; inhibition of ABCB1 elevated the BLI intensity two-fold only in HEK-293/rLuc cells. BLI of xenografts derived from HEK-293/ABC transporter/luciferase reporter cells confirmed the results of inhibitor treatment in vivo. These findings demonstrate that coelenterazine-based rLuc-BLI intensity can be modulated by ABCB1 and ABCG2. ABCG2 modulates d-luciferin-based BLI in a luciferase type-independent manner. Little ABC transporter effect on gLuc-BLI intensity is observed because a large fraction of gLuc is secreted. The expression level of ABC transporters is one key factor affecting BLI intensity, and this may be particularly important in luciferase-based applications in stem cell research.

摘要

生物发光成像(BLI)的荧光素酶报告基因提供了一种经济有效的和敏感的手段来成像生物过程。然而,荧光素酶底物的跨细胞膜转运确实会影响完整活细胞的 BLI 读出强度。为了研究 ABC 转运蛋白对 BLI 读出的影响,我们生成了具有不同 ABC 转运蛋白(ABCB1、ABCC1 和 ABCG2)过表达的叩头虫(cLuc)、萤火虫(fLuc)、海肾(rLuc)和高斯(gLuc)荧光素酶 HEK-293 报告细胞。体外研究表明,当 ABCG2 在 HEK-293/cLuc、fLuc 和 rLuc 细胞中过表达时,与细胞裂解物相比,完整细胞的 BLI 强度显著降低。还应用了选择性 ABC 转运蛋白抑制剂。ABCG2 活性的抑制使 HEK-293/cLuc、fLuc 和 rLuc 细胞的 BLI 强度增加了两倍以上;ABCB1 的抑制仅使 HEK-293/rLuc 细胞的 BLI 强度增加了两倍。来自 HEK-293/ABC 转运蛋白/荧光素酶报告细胞的异种移植物的 BLI 证实了体内抑制剂处理的结果。这些发现表明,腔肠素基 rLuc-BLI 强度可以被 ABCB1 和 ABCG2 调节。ABCG2 以与荧光素酶类型无关的方式调节 d-荧光素基 BLI。由于 gLuc 的很大一部分被分泌,因此对 gLuc-BLI 强度的 ABC 转运蛋白影响很小。ABC 转运蛋白的表达水平是影响 BLI 强度的一个关键因素,这在基于荧光素酶的干细胞研究应用中可能尤为重要。

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