Development of an Acute Method to Deliver Transgenes Into the Brains of Adult Xenopus laevis

Development of an Acute Method to Deliver Transgenes Into the Brains of Adult Xenopus laevis

The central vocal pathway of the African clawed frog, , is a powerful vertebrate model to understand mechanisms underlying central pattern generation. However, fast and efficient methods of introducing exogenous genes into the neurons of adult are currently not available. Here, we systematically tes...

Ausführliche Beschreibung

Gespeichert in:
Bibliographische Detailangaben
Veröffentlicht in:Frontiers in neural circuits 2018-10, Vol.12, p.92-92
Hauptverfasser: Yamaguchi, Ayako, Woller, Diana J, Rodrigues, Paulo
Format: Artikel
Sprache:eng
Schlagworte:
Age Factors
Animals
Axons
Brain
Brain - cytology
Brain - physiology
Brain Chemistry
Central nervous system
Electroporation
Electroporation - methods
Frogs
Gene expression
Gene Expression Regulation, Developmental
Gene Transfer Techniques
Genetic engineering
Genetic Vectors - administration & dosage
Genetic Vectors - genetics
Glycoproteins
Infections
Mammals
Membrane Glycoproteins - administration & dosage
Membrane Glycoproteins - genetics
Membrane Potentials - drug effects
Membrane Potentials - physiology
Methods
Neurogenesis
Neurons
Neuroscience
Neurosciences
Plasmids - administration & dosage
Plasmids - genetics
Rabies
Research programs
Stomatitis
Time Factors
transgene
Transgenes
Transgenes - physiology
Vectors (Biology)
vesicular stomatitis virus
Viral Envelope Proteins - administration & dosage
Viral Envelope Proteins - genetics
viral vector
Viruses
vocalizations
Xenopus
Xenopus laevis
Zebrafish
Online-Zugang:Volltext
Tags: Tag hinzufügen
Keine Tags, Fügen Sie den ersten Tag hinzu!
Beschreibung
Zusammenfassung:The central vocal pathway of the African clawed frog, , is a powerful vertebrate model to understand mechanisms underlying central pattern generation. However, fast and efficient methods of introducing exogenous genes into the neurons of adult are currently not available. Here, we systematically tested methods of transgene delivery into adult neurons. Although successfully used for tadpole neurons for over a decade, electroporation was not efficient in transfecting adult neurons. Similarly, adeno-associated virus (AAV) was not reliable, and lentivirus (LV) failed to function as viral vector in adult neurons. In contrast, vesicular stomatitis virus (VSV) was a fast and robust vector for adult neurons. Although toxic to the host cells, VSV appears to be less virulent to frog neurons than they are to mice neurons. At a single cell level, infected neurons showed normal physiological properties up to 7 days post infection and vocal circuits that included infected neurons generated normal fictive vocalizations up to 9 days post infection. The relatively long time window during which the physiology of VSV-infected neurons can be studied presents an ideal condition for the use of optogenetic tools. We showed that VSV does not gain entry into myelinated axons, but is taken up by both the soma and axon terminal; this is an attractive feature that drives transgene expression in projection neurons. Previous studies showed that VSVs can spread across synapses in anterograde or retrograde directions depending on the types of glycoprotein that are encoded. However, rVSV did not spread across synapses in the central nervous system. The successful use of VSV as a transgene vector in amphibian brains not only allows us to exploit the full potential of the genetic tools to answer questions central to understanding central pattern generation, but also opens the door to other research programs that focus on non-genetic model organisms to address unique questions.
ISSN:1662-5110
1662-5110
DOI:10.3389/fncir.2018.00092