Fibroblasts Can Be Genetically Modified to Produce Excitable Cells Capable of Electrical Coupling

Background—Cardiac conduction occurs in an electrical syncytium of excitable cells connected by gap junctions. Disruption of these electrophysiological properties causes conduction slowing or block. Depending on the location of affected cells within the heart, this has the potential to result in clinical syndromes such as atrioventricular block. With a view to developing gene therapy strategies for repairing cardiac conduction defects, we sought to establish whether the phenotype of fibroblasts can be modified by gene transfer to produce cells capable of electrical excitation and coupling. Methods and Results—High-titer lentiviral vectors encoding MyoD, a myogenic transcription factor, and connexin43, a gap junction protein, were produced by established methods. Human dermal fibroblasts (HDFs) were efficiently (>80%) transduced at a multiplicity of infection of 50. HDFs transduced with the MyoD-encoding vector underwent myogenic conversion, as evidenced by myotube formation and detection of muscle-specific proteins. Importantly, calcium transients indicative of membrane excitability were observed in MyoD-induced myotubes after loading with a calcium-sensitive dye and electrical stimulation. Transients from adjacent myotubes displayed different excitation thresholds, indicating an absence of coupling between cells, consistent with skeletal muscle biology. In contrast, simultaneous transduction of HDFs with MyoD and connexin43-encoding vectors resulted in the appearance of transients in adjacent myotubes with identical thresholds, indicative of electrical coupling. Notably, dye transfer studies confirmed gap junctional intercellular communication. Conclusions—Fibroblasts can be genetically modified to produce excitable cells capable of electrical coupling. These observations strengthen the prospect of developing gene-based strategies for repairing cardiac conduction defects.

[1]  D. Trono,et al.  A Third-Generation Lentivirus Vector with a Conditional Packaging System , 1998, Journal of Virology.

[2]  E. Kizana,et al.  Cardiac gene therapy: therapeutic potential and current progress. , 2003, Current gene therapy.

[3]  Michael R Rosen,et al.  Biological Pacemaker Implanted in Canine Left Bundle Branch Provides Ventricular Escape Rhythms That Have Physiologically Acceptable Rates , 2004, Circulation.

[4]  A. Kleber,et al.  Optical recording of impulse propagation in designer cultures. Cardiac tissue architectures inducing ultra-slow conduction. , 1999, Trends in cardiovascular medicine.

[5]  C. Antzelevitch Basic mechanisms of reentrant arrhythmias. , 2001, Current opinion in cardiology.

[6]  L. Ailles,et al.  Gene transfer by lentiviral vectors is limited by nuclear translocation and rescued by HIV-1 pol sequences , 2000, Nature Genetics.

[7]  E. Marbán,et al.  Focal modification of electrical conduction in the heart by viral gene transfer , 2000, Nature Medicine.

[8]  D. Allen,et al.  C2C12 co-culture on a fibroblast substratum enables sustained survival of contractile, highly differentiated myotubes with peripheral nuclei and adult fast myosin expression. , 2004, Cell motility and the cytoskeleton.

[9]  Y. Rudy The ionic mechanisms of conduction in cardiac tissue. , 2001, Journal of electrocardiology.

[10]  S. Marom,et al.  Electrophysiological Modulation of Cardiomyocytic Tissue by Transfected Fibroblasts Expressing Potassium Channels: A Novel Strategy to Manipulate Excitability , 2002, Circulation.

[11]  T. Hope,et al.  Woodchuck Hepatitis Virus Posttranscriptional Regulatory Element Enhances Expression of Transgenes Delivered by Retroviral Vectors , 1999, Journal of Virology.

[12]  L. Cronier,et al.  Involvement of gap junctional communication in myogenesis. , 2000, International review of cytology.

[13]  Michael R Rosen,et al.  Expression and Function of a Biological Pacemaker in Canine Heart , 2003, Circulation.

[14]  Y. Rudy,et al.  Basic mechanisms of cardiac impulse propagation and associated arrhythmias. , 2004, Physiological reviews.

[15]  I. Alexander,et al.  Adeno-associated virus and lentivirus vectors mediate efficient and sustained transduction of cultured mouse and human dorsal root ganglia sensory neurons. , 2001, Human gene therapy.