Literature DB >> 21248702

Direct delivery of MIF morpholinos into the zebrafish otocyst by injection and electroporation affects inner ear development.

Katie E Holmes1, Matthew J Wyatt, Yu-chi Shen, Deborah A Thompson, Kate F Barald.   

Abstract

In recent years, electroporation has become a popular technique for in vivo transfection of DNA, RNA, and morpholinos into various tissues, including the eye, brain, and somites of zebrafish. The advantage of electroporation over other methods of genetic manipulation is that specific tissues can be targeted, both spatially and temporally, for the introduction of macromolecules by the application of electrical current. Here we describe the use of electroporation for transfecting mif and mif-like morpholinos into the tissues of the developing inner ear of the zebrafish. In past studies, mif morpholino injected into embryos at the 1- to 8-cell stage resulted in widespread morphological changes in the nervous system and eye, as well as the ear. By targeting the tissues of the inner ear at later stages in development, we can determine the primary effects of MIF in the developing inner ear, as opposed to secondary effects that may result from the influence of other tissues. By using phalloidin and acetylated tubulin staining to study the morphology of neurons, neuronal processes, and hair cells associated with the posterior macula, we were able to assess the efficacy of electroporation as a method for targeted transfection in the zebrafish inner ear. The otic vesicles of 24hpf embryos were injected with morpholinos and electroporated and were then compared to embryos that had received no treatment or had been only injected or electroporated. Embryos that were injected and electroporated showed a decrease in hair cell numbers, decreased innervation by the statoacoustic ganglion (SAG) and fewer SAG neurons compared with control groups. Our results showed that direct delivery of morpholinos into otocysts at later stages avoids the non-specific nervous system and neural crest effects of morpholinos delivered at the 1-8 cell stage. It also allows examination of effects that are directed to the inner ear and not secondary effects on the ear from primary effects on the brain, neural crest or periotic mesenchyme.

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Year:  2011        PMID: 21248702      PMCID: PMC3182642          DOI: 10.3791/2466

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


  3 in total

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Journal:  J Biol Chem       Date:  2004-03-15       Impact factor: 5.157

  3 in total
  3 in total

1.  The cytokine macrophage migration inhibitory factor (MIF) acts as a neurotrophin in the developing inner ear of the zebrafish, Danio rerio.

Authors:  Yu-chi Shen; Deborah L Thompson; Meng-Kiat Kuah; Kah-Loon Wong; Karen L Wu; Stephanie A Linn; Ethan M Jewett; Alexander Chong Shu-Chien; Kate F Barald
Journal:  Dev Biol       Date:  2011-12-22       Impact factor: 3.582

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Journal:  Dev Dyn       Date:  2016-11-17       Impact factor: 3.780

3.  Macrophage migration inhibitory factor acts as a neurotrophin in the developing inner ear.

Authors:  Lisa M Bank; Lynne M Bianchi; Fumi Ebisu; Dov Lerman-Sinkoff; Elizabeth C Smiley; Yu-chi Shen; Poornapriya Ramamurthy; Deborah L Thompson; Therese M Roth; Christine R Beck; Matthew Flynn; Ryan S Teller; Luming Feng; G Nicholas Llewellyn; Brandon Holmes; Cyrrene Sharples; Jaeda Coutinho-Budd; Stephanie A Linn; Andrew P Chervenak; David F Dolan; Jennifer Benson; Ariane Kanicki; Catherine A Martin; Richard Altschuler; Alisa E Koch; Alicia E Koch; Ethan M Jewett; John A Germiller; Kate F Barald
Journal:  Development       Date:  2012-12       Impact factor: 6.868

  3 in total

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