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Analyzing Responses of Mouse Olfactory Sensory Neurons Using the Air-phase Electroolfactogram Recording


JoVE 1850 3/02/2010

Biology, Johns Hopkins University

The electroolfactogram (EOG) recording is an informative, easy-to-conduct, and reliable way of assessing olfactory function at the level of the olfactory epithelium. This protocol describes a recording setup, mouse tissue preparation, data collection, and basic data analysis.

 

Progressive-ratio Responding for Palatable High-fat and High-sugar Food in Mice


JoVE 3754 5/03/2012

CRCHUM and the Montreal Diabetes Research Center, University of Montreal

The present report details the protocol employed to measure the rewarding effects of high-fat food in mice using a progressive ratio operant conditioning task.

 

Visualization of DNA Replication in the Vertebrate Model System DT40 using the DNA Fiber Technique


JoVE 3255 10/27/2011

1Department of Molecular Oncology, Weatherall Institute of Molecular Medicine, University of Oxford , 2Institute of Genetics and Biotechnology, Faculty of Biology, University of Warsaw

DT40, a model vertebrate genetic system, provides a powerful tool to analyze protein function. Here we describe a simple method that allows qualitative analysis of parameters that influence DNA synthesis during the S-phase in DT40 cells at the single molecule level.

 

In utero and ex vivo Electroporation for Gene Expression in Mouse Retinal Ganglion Cells


JoVE 1333 9/24/2009

1Departments of Pathology and Cell Biology, and Neuroscience, Columbia University College of Physicians and Surgeons, 2Department of Ophthalmology, Columbia University College of Physicians and Surgeons

Here we present two techniques for manipulating gene expression in murine retinal ganglion cells (RGCs) by in utero and ex vivo electroporation. These techniques enable one to examine how alterations in gene expression affect RGC development, axon guidance, and functional properties.

 

Crystallizing Membrane Proteins for Structure Determination using Lipidic Mesophases


JoVE 1712 11/21/2010

Membrane Structural and Functional Biology Group, Schools of Biochemistry and Immunology and Medicine, Trinity College Dublin

Herein is described the procedure implemented in the Caffrey Membrane Structural and Functional Biology Group to set up manually crystallization trials of membrane proteins in lipidic mesophases.

 

Isolation of Translating Ribosomes Containing Peptidyl-tRNAs for Functional and Structural Analyses


JoVE 2498 2/25/2011

1Department of Biological Sciences, University of Alabama Huntsville, 2Department of Biology, Stanford University

A major impediment to biochemical analyses of ribosomes containing nascent peptidyl-tRNAs has been the presence of other ribosomes in the same samples, ribosomes not involved in the translation of the specific mRNA sequence being analyzed. We developed a simple methodology to purify, exclusively, the ribosomes containing the nascent peptidyl-tRNA of interest.

 

Preparation of Highly Coupled Rat Heart Mitochondria


JoVE 2202 9/23/2010

1Faculty of Life Sciences, University of Manchester, 2School of Biological Sciences, Queen's University Belfast

We describe а protocol for isolation of pure, highly coupled rat heart mitochondria for functional or structural studies of cellular bioenergetics, biophysical measurements, proteomics or mitochondrial DNA and lipids analysis.

 

Long-term Culture of Human Breast Cancer Specimens and Their Analysis Using Optical Projection Tomography


JoVE 3085 7/29/2011

1Breakthrough Breast Cancer Research Unit, Institute of Genetics and Molecular Medicine, University of Edinburgh, 2MRC Technology

We have developed a collagen-based in vitro assay which promotes proliferation and invasion from samples of all breast cancer subtypes. Optical Projection Tomography, a three dimensional microscopy technique was utilised to visualise and quantify tumour expansion. This assay may be used to quantify drug response of individual tumour samples.

 

Myo-mechanical Analysis of Isolated Skeletal Muscle


JoVE 2582 2/22/2011

1Cardiovascular Research Institute, University of California San Francisco, 2Department of Pediatrics, University of California San Francisco, 3Department of Biology, San Francisco State University, 4Department of Medicine, University of California San Francisco , 5Eli and Edythe Broad Center of Regeneration Medicine & Stem Cell Research, University of California San Francisco

To assess the in vivo effects of therapeutic interventions for muscle disease, methods are needed to quantitate force generation and fatigability in treated muscle. We detail an approach to evaluating myo-mechanical properties in explanted mouse hindlimb muscle. This analysis provides a robust approach to quantitating the effects of genetic modification on muscle function, as well as comparison of therapies in mouse models of muscle disease.

 

Generation of Neural Stem Cells from Discarded Human Fetal Cortical Tissue


JoVE 2681 5/25/2011

1Department of Neurology, Beth Israel Deaconess Medical Center, 2Department of Obstetrics and Gynecology, Brigham and Women's Hospital, 3Department of Pathology, Beth Israel Deaconess Medical Center, 4Department of Pathology, Division of Neuropathology, Brigham and Women's Hospital

A simple and reliable method on isolation and culture of neural stem cells from discarded human fetal cortical tissue is described. Cultures derived from known human neurological disorders can be used for characterization of pathological cellular and molecular processes, as well as provide a platform to assess pharmacological efficacy.

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