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基于突变型人雌激素受体的配体诱导分子内折叠的靶向基因治疗的可滴定两步转录扩增策略。

A titratable two-step transcriptional amplification strategy for targeted gene therapy based on ligand-induced intramolecular folding of a mutant human estrogen receptor.

作者信息

Chen Ian Y, Paulmurugan Ramasamy, Nielsen Carsten H, Wang David S, Chow Vinca, Robbins Robert C, Gambhir Sanjiv S

机构信息

Department of Medicine, Division of Cardiovascular Medicine, Stanford University School of Medicine, Stanford University, Stanford, CA, USA.

出版信息

Mol Imaging Biol. 2014 Apr;16(2):224-34. doi: 10.1007/s11307-013-0673-4.

Abstract

PURPOSE

The efficacy and safety of cardiac gene therapy depend critically on the level and the distribution of therapeutic gene expression following vector administration. We aimed to develop a titratable two-step transcriptional amplification (tTSTA) vector strategy, which allows modulation of transcriptionally targeted gene expression in the myocardium.

PROCEDURES

We constructed a tTSTA plasmid vector (pcTnT-tTSTA-fluc), which uses the cardiac troponin T (cTnT) promoter to drive the expression of the recombinant transcriptional activator GAL4-mER(LBD)-VP2, whose ability to transactivate the downstream firefly luciferase reporter gene (fluc) depends on the binding of its mutant estrogen receptor (ER(G521T)) ligand binding domain (LBD) to an ER ligand such as raloxifene. Mice underwent either intramyocardial or hydrodynamic tail vein (HTV) injection of pcTnT-tTSTA-fluc, followed by differential modulation of fluc expression with varying doses of intraperitoneal raloxifene prior to bioluminescence imaging to assess the kinetics of myocardial or hepatic fluc expression.

RESULTS

Intramyocardial injection of pcTnT-tTSTA-fluc followed by titration with intraperitoneal raloxifene led to up to tenfold induction of myocardial fluc expression. HTV injection of pcTnT-tTSTA-fluc led to negligible long-term hepatic fluc expression, regardless of the raloxifene dose given.

CONCLUSIONS

The tTSTA vector strategy can effectively modulate transgene expression in a tissue-specific manner. Further refinement of this strategy should help maximize the benefit-to-risk ratio of cardiac gene therapy.

摘要

目的

心脏基因治疗的疗效和安全性关键取决于载体给药后治疗性基因表达的水平和分布。我们旨在开发一种可滴定的两步转录扩增(tTSTA)载体策略,该策略能够调节心肌中转录靶向基因的表达。

程序

我们构建了一种tTSTA质粒载体(pcTnT-tTSTA-fluc),它利用心肌肌钙蛋白T(cTnT)启动子驱动重组转录激活因子GAL4-mER(LBD)-VP2的表达,其反式激活下游萤火虫荧光素酶报告基因(fluc)的能力取决于其突变雌激素受体(ER(G521T))配体结合域(LBD)与诸如雷洛昔芬等ER配体的结合。小鼠接受心肌内或尾静脉液压注射(HTV)pcTnT-tTSTA-fluc,然后在生物发光成像之前用不同剂量的腹腔内雷洛昔芬对fluc表达进行差异调节,以评估心肌或肝脏fluc表达的动力学。

结果

心肌内注射pcTnT-tTSTA-fluc后用腹腔内雷洛昔芬滴定导致心肌fluc表达诱导高达10倍。无论给予何种雷洛昔芬剂量,HTV注射pcTnT-tTSTA-fluc导致长期肝脏fluc表达可忽略不计。

结论

tTSTA载体策略能够以组织特异性方式有效调节转基因表达。对该策略的进一步优化应有助于使心脏基因治疗的风险效益比最大化。

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