Development of a lentivirus vector-based assay for non-destructive monitoring of cell fusion activity

Zeinab Neshati; Jia Liu; Guangqian Zhou; Martin J Schalij; Antoine A F de Vries

doi:10.1371/journal.pone.0102433

Development of a lentivirus vector-based assay for non-destructive monitoring of cell fusion activity

PLoS One. 2014 Jul 16;9(7):e102433. doi: 10.1371/journal.pone.0102433. eCollection 2014.

Authors

Zeinab Neshati¹, Jia Liu², Guangqian Zhou³, Martin J Schalij¹, Antoine A F de Vries¹

Affiliations

¹ Heart Center Leiden, Leiden University Medical Center, Leiden, The Netherlands.
² Heart Center Leiden, Leiden University Medical Center, Leiden, The Netherlands; Shenzhen University Medical School, Shenzhen University, Shenzhen, People's Republic of China.
³ Shenzhen University Medical School, Shenzhen University, Shenzhen, People's Republic of China.

Abstract

Cell-to-cell fusion can be quantified by endowing acceptor and donor cells with latent reporter genes/proteins and activators of these genes/proteins, respectively. One way to accomplish this goal is by using a bipartite lentivirus vector (LV)-based cell fusion assay system in which the cellular fusion partners are transduced with a flippase-activatable Photinus pyralis luciferase (PpLuc) expression unit (acceptor cells) or with a recombinant gene encoding FLPeNLS+, a nuclear-targeted and molecularly evolved version of flippase (donor cells). Fusion of both cell populations will lead to the FLPe-dependent generation of a functional PpLuc gene. PpLuc activity is typically measured in cell lysates, precluding consecutive analysis of one cell culture. Therefore, in this study the PpLuc-coding sequence was replaced by that of Gaussia princeps luciferase (GpLuc), a secretory protein allowing repeated analysis of the same cell culture. In myotubes the spread of FLPeNLS+ may be limited due to its nuclear localization signal (NLS) causing low signal outputs. To test this hypothesis, myoblasts were transduced with LVs encoding either FLPeNLS+ or an NLS-less version of FLPe (FLPeNLS-) and subsequently co-cultured in different ratios with myoblasts containing the FLPe-activatable GpLuc expression cassette. At different times after induction of cell-to-cell fusion the GpLuc activity in the culture medium was determined. FLPeNLS+ and FLPeNLS- both activated the latent GpLuc gene but when the percentage of FLPe-expressing myoblasts was limiting, FLPeNLS+ generally yielded slightly higher signals than FLPeNLS- while at low acceptor-to-donor cell ratios FLPeNLS- was usually superior. The ability of FLPeNLS+ to spread through myofibers and to induce reporter gene expression is thus not limited by its NLS. However, at high FLPe concentrations the presence of the NLS negatively affected reporter gene expression. In summary, a rapid and simple chemiluminescence assay for quantifying cell-to-cell fusion progression based on GpLuc has been developed.

Publication types

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

MeSH terms

Animals
Base Sequence
Blotting, Western
Cell Fusion / methods*
Fireflies / enzymology
Genes, Reporter / genetics*
Genetic Vectors / genetics*
Immunohistochemistry
Lentivirus
Luciferases / genetics
Luminescent Measurements / methods*
Mice
Molecular Sequence Data
Myoblasts / metabolism
Nuclear Localization Signals / metabolism
Oligodeoxyribonucleotides / genetics
Plasmids / genetics
Sequence Alignment

Substances

Nuclear Localization Signals
Oligodeoxyribonucleotides
Luciferases

Grants and funding

This work was supported by research grants from the Dutch Duchenne Parent Project (DPP) and the Iranian Ministry of Science, Research and Technology. The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.