logo
搜索
菜单

Intracerebroventricular and Intravascular Injection of Viral Particles and Fluorescent Microbeads into the Neonatal Brain

作者: Hideya Kawasaki1, Isao Kosugi1, Makiko Sakao-Suzuki2, Shiori Meguro1, Yoshihiro Tsutsui3, Toshihide Iwashita1 1Department of Regenerative & Infectious Pathology,Hamamatsu University School of Medicine, 2First Department of Medicine,Hamamatsu University School of Medicine, 3Faculty of Health Science,Tokoha University
简介:

Overview

This article describes a method for intracerebroventricular and intravascular injection of viral particles or fluorescent microbeads into the neonatal mouse brain. The technique allows for the observation of viral distribution during the acute phase of infection in the central nervous system.

Key Study Components

Area of Science

  • Neurovirology
  • Neuroscience
  • Infection dynamics

Background

  • Understanding viral distribution in the immature central nervous system is crucial.
  • Acute infection phases present unique challenges for observation.
  • Microscopic evaluation is essential for tracking viral particles.
  • Fluorescent microbeads can serve as a model for studying viral behavior.

Purpose of Study

  • To observe the distribution of viral particles in the neonatal mouse brain.
  • To answer key questions regarding viral behavior during infection.
  • To provide a straightforward method for researchers in neurovirology.

Methods Used

  • Sterilization of a 10 microliter syringe and a 27 gauge needle.
  • Intracerebroventricular injection of viral particles.
  • Intravascular injection of fluorescent microbeads.
  • Microscopic evaluation and in situ hybridization for localization.

Main Results

  • Direct observation of viral particle distribution is possible.
  • Both injection methods yield observable results under a microscope.
  • Initial distribution patterns can be effectively documented.
  • Insights into viral behavior during the acute phase of infection are gained.

Conclusions

  • The methods described are effective for studying viral distribution.
  • This approach can enhance understanding of neurovirology.
  • Future research can build on these findings to explore further questions.

Frequently Asked Questions

What is the main goal of this procedure?
The main goal is to observe the distribution of viral particles during the acute phase of infection in the central nervous system.
What are the advantages of this technique?
The technique allows for direct observation of viral particles using simple methods.
How are the syringes and needles prepared?
They are sterilized with 70% alcohol before use.
What types of particles can be injected?
Both viral particles and fluorescent microbeads can be injected.
What methods are used for localization?
Localization can be detected by microscopic evaluation or in situ hybridization.
Who can benefit from this study?
Researchers in the fields of neurovirology and neuroscience can benefit from this study.

Here, we describe a simple method of intracerebroventricular and intravascular injection of viral particles or fluorescent microbeads into the neonatal mouse brain. The localization pattern of the virus and nanoparticles could be detected by microscopic evaluation or by in situ hybridization.

标签: Intracerebroventricular,    Intravascular,    Viral Particles,    Fluorescent Microbeads,    Neonatal Brain,    Murine Cytomegalovirus,    Lateral Ventricle,    Superficial Temporal Vein,    Neurovirology,    Acute Infection Phase,    Virus Distribution,    Microscopy,    Injection,    Anesthesia,    Neonatal Mouse,   
Quantitative Measurement of Relative Retinoic Acid Levels in E8.5 Embryos and Neurosphere Cultures Using the F9 RARE-Lacz Cell-based Reporter Assay 10.3791/54443-v
Quantitative Measurement of Relative Retinoic Acid Levels in E8.5 Embryos and Neurosphere Cultures Using the F9 RARE-Lacz Cell-based Reporter Assay
Taste Preference Assay for Adult Drosophila 10.3791/54403-v 04:31 min
Taste Preference Assay for Adult Drosophila
Fabrication of High Contact-Density, Flat-Interface Nerve Electrodes for Recording and Stimulation Applications 10.3791/54388-v 09:35 min
Fabrication of High Contact-Density, Flat-Interface Nerve Electrodes for Recording and Stimulation Applications
Automated Analysis of C. elegans Swim Behavior Using CeleST Software 10.3791/54359-v
Automated Analysis of C. elegans Swim Behavior Using CeleST Software
Fluorescence Activated Cell Sorting (FACS) and Gene Expression Analysis of Fos-expressing Neurons from Fresh and Frozen Rat Brain Tissue 10.3791/54358-v 08:37 min
Fluorescence Activated Cell Sorting (FACS) and Gene Expression Analysis of Fos-expressing Neurons from Fresh and Frozen Rat Brain Tissue
External Excitation of Neurons Using Electric and Magnetic Fields in One- and Two-dimensional Cultures 10.3791/54357-v 08:32 min
External Excitation of Neurons Using Electric and Magnetic Fields in One- and Two-dimensional Cultures
Protocol for Isolating the Mouse Circle of Willis 10.3791/54352-v 06:30 min
Protocol for Isolating the Mouse Circle of Willis
SNARE-mediated Fusion of Single Proteoliposomes with Tethered Supported Bilayers in a Microfluidic Flow Cell Monitored by Polarized TIRF Microscopy 10.3791/54349-v 10:58 min
SNARE-mediated Fusion of Single Proteoliposomes with Tethered Supported Bilayers in a Microfluidic Flow Cell Monitored by Polarized TIRF Microscopy
返回顶部