Dissection of the Adult Zebrafish Kidney

JoVE 2839 8/29/2011

Gary F. Gerlach*, Lauran N. Schrader*, Rebecca A. Wingert

Department of Biological Sciences, University of Notre Dame

The zebrafish kidney is home to both renal and hematopoietic adult stem/progenitor cells, and represents an outstanding opportunity to study these cell types and their progeny in a vertebrate model organism. Here, we demonstrate a detailed dissection procedure that enables the researcher to identify and surgically remove the adult zebrafish kidney, which can be used for applications such as cell isolation, transplantation, and expression studies of kidney and/or blood cell populations.

Assessing Teratogenic Changes in a Zebrafish Model of Fetal Alcohol Exposure

JoVE 3704 3/20/2012

Evyn Loucks¹, Sara Ahlgren^1,2

¹Program in Developmental Biology, Children's Memorial Research Center, ²Department of Pediatrics, Northwestern University

In order to understand the molecular mechanisms of the ethanol-induced developmental damage, we have developed a zebrafish model of ethanol exposure and are exploring the physical, cellular, and genetic alterations that occur after ethanol exposure¹. We then seek to find potential interventions and rapidly test them in this animal model.

Induction of Myocardial Infarction in Adult Zebrafish Using Cryoinjury

JoVE 3666 4/18/2012

Fabian Chablais, Anna Jaźwińska

Department of Biology, Unit of Zoology, University of Fribourg, Fribourg, Switzerland

Zebrafish represents a valuable model to study the mechanisms of heart regeneration in vertebrates. Here, we present a protocol for induction of a heart infarct in adult zebrafish using cryoinjury. This method results in massive cell death within 20% of the ventricular wall, similar to that observed in mammalian infarcts.

Whole Mount RNA Fluorescent in situ Hybridization of Drosophila Embryos

JoVE 50057 1/30/2013

Félix Legendre*^1,2, Neal Cody*¹, Carole Iampietro¹, Julie Bergalet¹, Fabio Alexis Lefebvre^1,2, Gaël Moquin-Beaudry^1,2, Olivia Zhang¹, Xiaofeng Wang¹, Eric Lécuyer^1,2

¹Institut de Recherches Cliniques de Montréal (IRCM), ²Department of Biochemistry, Université de Montréal

Here we describe a whole-mount fluorescent in situ hybridization (FISH) protocol for determining the expression and localization properties of RNAs expressed during embryogenesis in the fruit fly, Drosophila melanogaster.

Direct Delivery of MIF Morpholinos Into the Zebrafish Otocyst by Injection and Electroporation Affects Inner Ear Development

JoVE 2466 1/07/2011

Katie E. Holmes¹, Matthew J. Wyatt², Yu-chi Shen², Deborah A. Thompson^2,3, Kate F. Barald^2,4

¹Department of Veterinary Science, University of Wisconsin, Madison, ²Department of Cell and Developmental Biology, University of Michigan, Ann Arbor, MI, ³Present address: Department of Pulmonary Medicine, University of Michigan, Ann Arbor, MI, ⁴Department of Biomedical Engineering, University of Michigan, Ann Arbor, MI

A method to deliver morpholinos directly into the zebrafish otocyst at 24hpf has been developed. Using microinjection of morpholinos into the lumen of otic vesicle and electroporation to effect penetration, we were able to bypass the effect of morpholinos on the brain and obtain effects specific to the inner ear.

Hybridization in situ of Salivary Glands, Ovaries, and Embryos of Vector Mosquitoes

JoVE 3709 6/28/2012

Jennifer Juhn¹, Anthony A. James^1,2

¹Department of Molecular Biology and Biochemistry, University of California, Irvine, ²Department of Microbiology and Molecular Genetics, University of California, Irvine

Temporal and spatial gene expression analyses have a crucial role in functional genomics. Whole-mount hybridization in situ is useful for determining the localization of transcripts within tissues and subcellular compartments. Here we outline a hybridization in situ protocol with modifications for specific target tissues in mosquitoes.

Assay for Neural Induction in the Chick Embryo

JoVE 1027 2/13/2009

Delphine Psychoyos, Richard Finnell

Institute of Biosciences and Technology, Center for Environmental and Genetic Medicine, Texas A&M University (TAMU)

Neural induction is the first step in the formation of the brain. It is a mechanism by which Hensen's node (organizer), instructs adjacent tissue to adopt a neural fate, i.e. to give rise to the nervous system. This video demonstrates an assay for neural induction in chick embryo.

Radioactive in situ Hybridization for Detecting Diverse Gene Expression Patterns in Tissue

JoVE 3764 4/27/2012

Chun-Chun Chen¹, Kazuhiro Wada², Erich D. Jarvis¹

¹Howard Hughes Medical Institute, Department of Neurobiology, Duke University, ²Department of Biological Sciences, Hokkaido University

This protocol is successfully used to quantitatively detect levels and spatial patterns of mRNA expression in multiple tissue types across vertebrate species. The method can detect low abundance transcripts and allows processing of hundreds of slides simultaneously. We present this protocol using expression profiling of avian embryonic brain formation as an example.

Chromosomal Spread Preparation of Human Embryonic Stem Cells for Karyotyping

JoVE 1512 9/04/2009

Priscila B. Campos, Rafaela C. Sartore, Stacie N. Abdalla, Stevens K. Rehen

Institute of Biomedical Sciences, Federal University of Rio De Janeiro-UFRJ

Karyotyping is a simple and useful technique widely used for detecting genetic alterations. Here we describe a step by step protocol for chromosome spread preparation of human embryonic stem cells for monitoring the chromosomal status of these cells maintained in culture.

In Situ Hybridization for the Precise Localization of Transcripts in Plants

JoVE 3328 11/23/2011

Marie Javelle, Cristina F. Marco, Marja Timmermans

Cold Spring Harbor Laboratory

The in situ hybridization protocol described here allows a direct localization of mRNA and small RNA expression at the cellular level with high sensitivity and specificity. The procedure is optimized for paraffin-embedded plant tissue sections, is applicable to a wide range of plants and tissues, and can be completed within ten days.

A Technique to Simultaneously Visualize Virus-Specific CD8+ T Cells and Virus-Infected Cells In situ

JoVE 1561 8/13/2009

Qingsheng Li¹, Pamela J. Skinner², Lijie Duan¹, Ashley T. Haase¹

¹Department of Microbiology, Medical School, University of Minnesota, ²Department of Veterinary and Biomedical Sciences, University of Minnesota

A technique combining in situ tetramer staining and in situ hybridization (ISTH) enables visualization, mapping and analysis of the spatial proximity of virus-specific CD8+ T cells to their virus-infected targets, and determination of the quantitative relationships between these immune effectors and targets to infection outcomes.

Analysis of mRNA Nuclear Export Kinetics in Mammalian Cells by Microinjection

JoVE 2387 12/04/2010

Serge Gueroussov, Stefan P. Tarnawsky, Xianying A. Cui, Kohila Mahadevan, Alexander F. Palazzo

Department of Biochemistry, University of Toronto

Here we describe an assay that employs the power of microinjection coupled with fluorescent in situ hybridization in order to accurately measure the nuclear export kinetics of mRNA in mammalian somatic cells.

Zebrafish Whole Mount High-Resolution Double Fluorescent In Situ Hybridization

JoVE 1229 3/25/2009

Tim Brend, Scott A. Holley

Department of Molecular, Cellular and Developmental Biology, Yale University

Whole mount in situ hybridization is one of the most widely used techniques in developmental biology. Here, we present a high-resolution double fluorescent in situ hybridization protocol for analyzing the precise expression pattern of a single gene and for determining the overlap of the expression domains of two genes. We include a propidium iodide nuclear counter-stain to highlight tissue organization.

Cell Block Preparation from Cytology Specimen with Predominance of Individually Scattered Cells

JoVE 1316 7/21/2009

George M. Varsegi, Vinod Shidham

Department of Pathology, University of Wisconsin - Milwaukee

Shidham's method for preparation of cell blocks with AV-marker from cytology specimens containing individually scattered cells and small cell groups.

Combining Lipophilic dye, in situ Hybridization, Immunohistochemistry, and Histology

JoVE 2451 3/17/2011

Jeremy Duncan¹, Jennifer Kersigo¹, Brian Gray², Bernd Fritzsch¹

¹Department of Biology, University of Iowa, ²Molecular Targeting Technologies, Inc.

A combination of different techniques to maximize data collection from mouse tissue is presented.

Whole Mount in Situ Hybridization of E8.5 to E11.5 Mouse Embryos

JoVE 2797 10/10/2011

Qiaozhi Wei, Nancy R. Manley, Brian G. Condie

Department of Genetics, University of Georgia

This whole mount in situ hybridization protocol discusses critical steps that ensure reproducible high quality results for gene expression studies in E8.5-E11.5 day old mouse embryos.

Methods for the Study of the Zebrafish Maxillary Barbel

JoVE 1558 11/23/2009

Elizabeth E. LeClair¹, Jacek Topczewski²

¹Department of Biological Sciences, DePaul University, ²Children’s Memorial Research Center, Department of Pediatrics, Northwestern University Feinberg School of Medicine

The zebrafish maxillary barbel is an integumentary sense organ containing ectodermal, mesodermal and neural crest derivatives. Importantly, the adult barbel can regenerate after proximal amputation. This video introduces maxillary barbel development and demonstrates a surgical protocol to induce regeneration, followed by collection, embedding and downstream imaging of barbel specimens.

Assessing Signaling Properties of Ectodermal Epithelia During Craniofacial Development

JoVE 2557 3/24/2011

Diane Hu, Ralph S. Marcucio

Department of Orthopaedic Surgery, University of California San Francisco

This article describes a tissue transplantation technique that was designed to test the signaling and patterning properties of surface cephalic ectoderm during craniofacial development.

High-throughput Physical Mapping of Chromosomes using Automated in situ Hybridization

JoVE 4007 6/28/2012

Phillip George, Maria V. Sharakhova, Igor V. Sharakhov

Department of Entomology, Virginia Tech

Genome assemblies based on massively parallel DNA sequencing technologies are usually highly fragmented. The development of physical chromosome maps can potentially improve genome assemblies. Here, we demonstrate innovative approaches to chromosome preparation, fluorescent in situ hybridization, and imaging that significantly increase throughput of the physical map development.

Blastomere Explants to Test for Cell Fate Commitment During Embryonic Development

JoVE 4458 1/26/2013

Paaqua A. Grant¹, Mona B. Herold¹, Sally A. Moody²

¹Department of Biological Sciences, The George Washington University, ²Department of Anatomy and Regenerative Biology, The George Washington University

The fate of an individual embryonic cell can be influenced by inherited molecules and/or by signals from neighboring cells. Utilizing fate maps of the cleavage stage Xenopus embryo, single blastomeres can be identified for culture in isolation to assess the contributions of inherited molecules versus cell-cell interactions.

Heart Dissection in Larval, Juvenile and Adult Zebrafish, Danio rerio

JoVE 3165 9/30/2011

Corinna Singleman, Nathalia G. Holtzman

Department of Biology, Queens College, City University of New York

A clear, standardized method for dissection and isolation of the zebrafish heart at multiple developmental stages are described. Annotation and quantification techniques are also discussed.

June 2012: This Month in JoVE

JoVE 4467 6/01/2012

Wendy Chao¹, Aaron Kolski-Andreaco²

¹Department of Ophthalmology, Massachusetts Eye and Ear, ²JoVE Content Production

Back in 1905, in what is now the Czech Republic, Eduard Zirm performed the first corneal transplantation surgery (keratoplasty), which restored vision to a patient blinded by corneal injury. Today, eye banks all over the world prepare, store, and distribute donated corneas to hospitals so that thousands of sight-saving keratoplasties can be performed every year. In June 2012, JoVE has its eye on two research groups, one from Italy and the other from Michigan, who demonstrate two distinct methods for corneal graft preparation prior to transplantation.

RNA In situ Hybridization in Whole Mount Embryos and Cell Histology Adapted for Marine Elasmobranchs

JoVE 50165 4/12/2013

Nicole A. Theodosiou

Department of Biological Sciences, Union College

By combining methods for RNA whole mount in situ hybridization and histology, gene expression can be linked with cell fate decisions in the developing embryo. These methods have been adapted to marine elasmobranchs and facilitate the use of these animals as model organisms for biomedical, toxicology and comparative studies.

Imaging Glycans in Zebrafish Embryos by Metabolic Labeling and Bioorthogonal Click Chemistry

JoVE 2686 6/06/2011

Hao Jiang¹, Lei Feng¹, David Soriano del Amo¹, Ronald D. Seidel III², Florence Marlow³, Peng Wu¹

¹Department of Biochemistry, Albert Einstein College of Medicine, Yeshiva University, ²Macromolecular Therapeutics Development Facility, Albert Einstein College of Medicine, Yeshiva University, ³Developmental and Molecular Biology, Albert Einstein College of Medicine, Yeshiva University

A click-chemistry based method that allows for the rapid, noninvasive, and robust labeling of alkyne-tagged glycans in zebrafish embryos is described. Fucosylated glycans in the enveloping layer of zebrafish embryos in the late gastrulation stage were imaged in this study.

A High Throughput in situ Hybridization Method to Characterize mRNA Expression Patterns in the Fetal Mouse Lower Urogenital Tract

JoVE 2912 8/19/2011

Lisa L. Abler, Vatsal Mehta, Kimberly P. Keil, Pinak S. Joshi, Chelsea-Leigh Flucus, Heather A. Hardin, Christopher T. Schmitz, Chad M. Vezina

Department of Comparative Biosciences, School of Veterinary Medicine, University of Wisconsin-Madison

Here, we describe an efficient high throughput in situ hybridization (ISH) method for visualizing patterns of mRNA expression in developing fetal mouse prostate tissue sections. The method can be easily adapted to visualize mRNA expression patterns in other mouse tissues or in tissues from other species.

Using Whole Mount in situ Hybridization to Link Molecular and Organismal Biology

JoVE 2533 3/31/2011

Nicole L. Jacobs¹, R. Craig Albertson¹, Jason R. Wiles^1,2

¹Department of Biology, Syracuse University, ²Department of Science Teaching, Syracuse University

Whole mount in situ hybridization (WISH) was used in an upper level undergraduate Comparative Vertebrate Biology course in addition to vertebrate dissections. This gave students the opportunity to study gene expression patterns as well as gross anatomy, linking the study of molecular and organismal biology within one course.

Dissection of Drosophila Ovaries

JoVE 52 10/19/2006

Li Chin Wong, Paul Schedl

Princeton University