Literature DB >> 21694690

The mouse cremaster muscle preparation for intravital imaging of the microcirculation.

Pooneh Bagher1, Steven S Segal.   

Abstract

Throughout the body, the maintenance of homeostasis requires the constant supply of oxygen and nutrients concomitant with removal of metabolic by-products. This balance is achieved by the movement of blood through the microcirculation, which encompasses the smallest branches of the vascular supply throughout all tissues and organs. Arterioles branch from arteries to form networks that control the distribution and magnitude of oxygenated blood flowing into the multitude of capillaries intimately associated with parenchymal cells. Capillaries provide a large surface area for diffusional exchange between tissue cells and the blood supply. Venules collect capillary effluent and converge as they return deoxygenated blood towards the heart. To observe these processes in real time requires an experimental approach for visualizing and manipulating the living microcirculation. The cremaster muscle of rats was first used as a model for studying inflammation using histology and electron microscopy post mortem. The first in vivo report of the exposed intact rat cremaster muscle investigated microvascular responses to vasoactive drugs using reflected light. However curvature of the muscle and lack of focused illumination limited the usefulness of this preparation. The major breakthrough entailed opening the muscle, detaching it from the testicle and spreading it radially as a flat sheet for transillumination under a compound microscope. While shown to be a valuable preparation to study the physiology of the microcirculation in rats and hamsters, the cremaster muscle in mice has proven particularly useful in dissecting cellular pathways involved in regulating microvascular function and real-time imaging of intercellular signaling. The cremaster muscle is derived from the internal oblique and transverse abdominus muscles as the testes descend through the inguinal canal. It serves to support (Greek: cremaster = suspender) and maintain temperature of the testes. As described here, the cremaster muscle is prepared as a thin flat sheet for outstanding optical resolution. With the mouse maintained at a stable body temperature and plane of anesthesia, surgical preparation involves freeing the muscle from surrounding tissue and the testes, spreading it onto transparent pedestal of silastic rubber and securing the edges with insect pins while irrigating it continuously with physiological salt solution. The present protocol utilizes transgenic mice expressing GCaMP2 in arteriolar endothelial cells. GCaMP2 is a genetically encoded fluorescent calcium indicator molecule. Widefield imaging and an intensified charge-coupled device camera enable in vivo study of calcium signaling in the arteriolar endothelium.

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Year:  2011        PMID: 21694690      PMCID: PMC3132939          DOI: 10.3791/2874

Source DB:  PubMed          Journal:  J Vis Exp        ISSN: 1940-087X            Impact factor:   1.355


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  22 in total

1.  Intravital microscopy of the microcirculation in the mouse cremaster muscle for the analysis of peripheral stem cell migration.

Authors:  Peter Donndorf; Marion Ludwig; Fabian Wildschütz; Dritan Useini; Alexander Kaminski; Brigitte Vollmar; Gustav Steinhoff
Journal:  J Vis Exp       Date:  2013-11-05       Impact factor: 1.355

2.  Blunted temporal activity of microvascular perfusion heterogeneity in metabolic syndrome: a new attractor for peripheral vascular disease?

Authors:  Joshua T Butcher; Adam G Goodwill; Shyla C Stanley; Jefferson C Frisbee
Journal:  Am J Physiol Heart Circ Physiol       Date:  2012-12-21       Impact factor: 4.733

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Authors:  Ian M Williams; Francisco A Valenzuela; Steven D Kahl; Doraiswami Ramkrishna; Adam R Mezo; Jamey D Young; K Sam Wells; David H Wasserman
Journal:  J Clin Invest       Date:  2018-01-08       Impact factor: 14.808

4.  The pulmonary endothelial glycocalyx regulates neutrophil adhesion and lung injury during experimental sepsis.

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Authors:  Brian Glancy; Li-Yueh Hsu; Lam Dao; Matthew Bakalar; Stephanie French; David J Chess; Joni L Taylor; Martin Picard; Angel Aponte; Mathew P Daniels; Shervin Esfahani; Samuel Cushman; Robert S Balaban
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6.  Microhemodynamic parameters quantification from intravital microscopy videos.

Authors:  Daniel Ortiz; Juan Carlos Briceño; Pedro Cabrales
Journal:  Physiol Meas       Date:  2014-01-30       Impact factor: 2.833

7.  Intravital investigation of rat mesenteric small artery tone and blood flow.

Authors:  Jakob Nyvad; Aleksandra Mazur; Dmitry D Postnov; Marthe Simonsen Straarup; Asger Maare Soendergaard; Christian Staehr; Emil Brøndum; Christian Aalkjaer; Vladimir V Matchkov
Journal:  J Physiol       Date:  2017-06-30       Impact factor: 5.182

8.  Interleukin-17A Promotes Aortic Endothelial Cell Activation via Transcriptionally and Post-translationally Activating p38 Mitogen-activated Protein Kinase (MAPK) Pathway.

Authors:  Jietang Mai; Gayani Nanayakkara; Jahaira Lopez-Pastrana; Xinyuan Li; Ya-Feng Li; Xin Wang; Ai Song; Anthony Virtue; Ying Shao; Huimin Shan; Fang Liu; Michael V Autieri; Satya P Kunapuli; Yoichiro Iwakura; Xiaohua Jiang; Hong Wang; Xiao-Feng Yang
Journal:  J Biol Chem       Date:  2016-01-05       Impact factor: 5.157

9.  Mitochondrial Reactive Oxygen Species Mediate Lysophosphatidylcholine-Induced Endothelial Cell Activation.

Authors:  Xinyuan Li; Pu Fang; Yafeng Li; Yin-Ming Kuo; Andrew J Andrews; Gayani Nanayakkara; Candice Johnson; Hangfei Fu; Huimin Shan; Fuyong Du; Nicholas E Hoffman; Daohai Yu; Satoru Eguchi; Muniswamy Madesh; Walter J Koch; Jianxin Sun; Xiaohua Jiang; Hong Wang; Xiaofeng Yang
Journal:  Arterioscler Thromb Vasc Biol       Date:  2016-04-28       Impact factor: 8.311

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Journal:  J Vasc Res       Date:  2015       Impact factor: 1.934

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