Truncated active human matrix metalloproteinase-8 delivered by a chimeric adenovirus-hepatitis B virus vector ameliorates rat liver cirrhosis

Jinxia Liu; Xin Cheng; Zhengrong Guo; Zihua Wang; Dong Li; Fubiao Kang; Haijun Li; Baosheng Li; Zhichen Cao; Michael Nassal; Dianxing Sun

doi:10.1371/journal.pone.0053392

Truncated active human matrix metalloproteinase-8 delivered by a chimeric adenovirus-hepatitis B virus vector ameliorates rat liver cirrhosis

PLoS One. 2013;8(1):e53392. doi: 10.1371/journal.pone.0053392. Epub 2013 Jan 3.

Authors

Jinxia Liu¹, Xin Cheng, Zhengrong Guo, Zihua Wang, Dong Li, Fubiao Kang, Haijun Li, Baosheng Li, Zhichen Cao, Michael Nassal, Dianxing Sun

Affiliation

¹ The Liver Diseases Diagnosis and Treatment Center of PLA, Bethune International Peace Hospital, Shijiazhuang, People's Republic of China.

Abstract

Background: Liver cirrhosis is a potentially life-threatening disease caused by progressive displacement of functional hepatocytes by fibrous tissue. The underlying fibrosis is often driven by chronic infection with hepatitis B virus (HBV). Matrix metalloproteinases including MMP-8 are crucial for excess collagen degradation. In a rat model of liver cirrhosis, MMP-8 delivery by an adenovirus (Ad) vector achieved significant amelioration of fibrosis but application of Ad vectors in humans is subject to various issues, including a lack of intrinsic liver specificity.

Methods: HBV is highly liver-specific and its principal suitability as liver-specific gene transfer vector is established. HBV vectors have a limited insertion capacity and are replication-defective. Conversely, in an HBV infected cell vector replication may be rescued in trans by the resident virus, allowing conditional vector amplification and spreading. Capitalizing on a resident pathogen to help in its elimination and/or in treating its pathogenic consequences would provide a novel strategy. However, resident HBV may also reduce susceptibility to HBV vector superinfection. Thus a size-compatible truncated MMP-8 (tMMP8) gene was cloned into an HBV vector which was then used to generate a chimeric Ad-HBV shuttle vector that is not subject to superinfection exclusion. Rats with thioacetamide-induced liver cirrhosis were injected with the chimera to evaluate therapeutic efficacy.

Results: Our data demonstrate that infectious HBV vector particles can be obtained via trans-complementation by wild-type virus, and that the tMMP8 HBV vector can efficiently be shuttled by an Ad vector into cirrhotic rat livers. There it exerted a comparable beneficial effect on fibrosis and hepatocyte proliferation markers as a conventional full-length MMP-8Ad vector.

Conclusions: Though the rat cirrhosis model does not allow assessing in vivo HBV vector amplification these results advocate the further development of Ad-HBV vectors for liver-specific gene therapy, including and perhaps particularly for HBV-related disease.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Adenoviridae / genetics*
Animals
Cell Proliferation
Collagen / metabolism
Disease Models, Animal
Fibrosis
Genetic Therapy / methods*
Genetic Vectors / genetics
Hep G2 Cells
Hepatitis B virus / genetics*
Hepatocytes / cytology
Humans
Liver / metabolism*
Liver Cirrhosis / metabolism
Liver Cirrhosis / therapy*
Matrix Metalloproteinase 8 / metabolism
Matrix Metalloproteinase 8 / therapeutic use*
Microscopy, Fluorescence
Rats
Transfection

Substances

Collagen
MMP8 protein, human
Matrix Metalloproteinase 8

Grants and funding

This work was supported by National Natural Science Foundation of China (grant numbers: 30872255; 30571667, URL of the funder’s website, http://isisn.nsfc.gov.cn/egrantweb/) and Chinese Foundation for Hepatitis Prevention and Control, Wang Baoen Liver Fibrosis Foundation (grant number: 20070001, URL of funder’s website, http://www.wbelff.org/keti.php). The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.