Distribution of immunoreactive alpha- and beta-subunit isoforms of Na,K-ATPase in the gerbil inner ear.

McGuirt, Joan P.; Schulte, Bradley A.

doi:10.1177/42.7.8014467

Cited by 70 publications

(53 citation statements)

References 25 publications

(37 reference statements)

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“…A comparison of the immunostaining pattern for NKCC1 with previous data mapping the distribution of the Na,K-ATPase pump and its isoforms in inner ear tissues (McGuirt and Schulte 1994;Schulte and Steel 1994), indicates the co-localization of these two ion transport mediators in distinct subsets of inner ear fibrocytes. On the basis of their location and gap junctional connections with other cell types, these specialized fibrocytes comprise the initial segments of syncytial cellular networks believed to have evolved for resorbing K ϩ leaked or effluxed from endolymph through hair cell activity and releasing it near epithelial cells for recycling back to endolymph (Schulte and Steel 1994;Spicer and Schulte 1996).…”

Section: Discussionmentioning

confidence: 99%

Immunohistochemical Localization of the Na-K-Cl Co-transporter (NKCC1) in the Gerbil Inner Ear

Crouch

Sakaguchi

Lytle

et al. 1997

J Histochem Cytochem.

165

133

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SUMMARYWe mapped the cellular and subcellular distribution of the Na-K-Cl co-transporter (NKCC) in the adult gerbil inner ear by immunostaining with a monoclonal antibody (MAb T4) generated against human colon NKCC. Heavy immunolabeling was seen in the basolateral plasma membrane of marginal cells in the stria vascularis and dark cells in the vestibular system. Subpopulations of fibrocytes in the cochlear spiral ligament and limbus and underlying the vestibular neurosensory epithelium also stained with moderate to strong intensity, apparently along their entire plasmalemma. Because MAb T4 recognizes both the basolateral secretory (NKCC1) and the apical absorptive (NKCC2) isoforms of the co-transporter, we employed reverse transcription and the polymerase chain reaction (RT-PCR) to explore isoform diversity in inner ear tissues. Using NKCC1 and NKCC2 isoform-specific PCR primers based on mouse and human sequences, only transcripts for NKCC1 were detected in the gerbil inner ear. The presence of abundant NKCC1 in the basolateral plasmalemma of strial marginal and vestibular dark cells confirms conclusions drawn from pharmacological and physiological data. The co-expression of NKCC1 and Na,K-ATPase in highly specialized subpopulations of cochlear and vestibular fibrocytes provides further evidence for their role in recycling K ϩ leaked or effluxed through hair cells into perilymph back to endolymph, as postulated in current models of inner ear ion homeostasis.

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Section: Discussionmentioning

confidence: 99%

Immunohistochemical Localization of the Na-K-Cl Co-transporter (NKCC1) in the Gerbil Inner Ear

Crouch

Sakaguchi

Lytle

et al. 1997

J Histochem Cytochem.

165

133

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“…In humans and rodents, the major expression sites of the ␤2 gene are brain (Shyjan et al, 1990a), pineal gland (Shyjan et al, 1990b), eye (Schneider et al, 1991), and ear (McGuirt and Schulte, 1994;Schulte and Steel, 1994). Together, the expression patterns for atp1b2a and atp1b2b closely parallel that seen for the single mammalian ␤2 gene.…”

Section: Resultsmentioning

confidence: 51%

Two Na,K-ATPase β2 subunit isoforms are differentially expressed within the central nervous system and sensory organs during zebrafish embryogenesis

Rajarao¹,

Canfield²,

Loppin³

et al. 2002

Dev. Dyn.

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We have identified cDNAs encoding a second zebrafish ortholog of the human Na,K-ATPase ␤2 subunit. The ␤2b cDNA encodes a 292 amino acid-long polypeptide with 74% identity to the previously characterized zebrafish ␤2a subunit. By using a zebrafish meiotic mapping panel, we determined that the ␤2b gene (atp1b2b) was tightly linked to markers on linkage group 5, whereas the ␤2a gene was located on linkage group 23. In situ hybridization analysis shows that in developing zebrafish embryos, atp1b2a and atp1b2b are predominantly expressed in the nervous system. ␤2a transcripts were abundantly expressed throughout brain as well as spinal cord neurons and lateral line ganglia. In contrast, ␤2b mRNA expression was primarily detected in sensory organs, including retina, otic vesicles, and lateral line neuromast cells. These results suggest that the ␤2a and ␤2b genes play distinct roles in developing brain and sensory organs, and raise the possibility that the functions encoded by the single mammalian ␤2 gene may be partitioned between the two zebrafish ␤2 orthologs.

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“…The distribution of VC 1.1 antigen and associated proteoglycan corresponded precisely with that of Na,K-ATPase and Na+ channels in nodes of Ranvier [24,32] and on the surface of neurons in the nucleus of the eighth nerve root [16]; and VC1.1 unaccompanied by proteoglycan colocalized with Na,KATPase on unmyelinated afferent terminals beneath cochlear and vestibular hair cells [23,27]. Moreover, the VC 1.1 epitope shown to occur as a constituent of chondroitin 6-SO4 proteoglycan on rod outer segments occurs at the site where Na+ channels function importantly in the response to light [21].…”

Section: Differentiation Of Glycoconjugates In Thementioning

confidence: 93%

Abundance and Diversity of Glycoconjugates Visualized Cytochemically in the Nervous System.

Spicer

Schulte

1995

Acta Histochem. Cytochem

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Distribution of immunoreactive alpha- and beta-subunit isoforms of Na,K-ATPase in the gerbil inner ear.

Cited by 70 publications

References 25 publications

Immunohistochemical Localization of the Na-K-Cl Co-transporter (NKCC1) in the Gerbil Inner Ear

Immunohistochemical Localization of the Na-K-Cl Co-transporter (NKCC1) in the Gerbil Inner Ear

Two Na,K-ATPase β2 subunit isoforms are differentially expressed within the central nervous system and sensory organs during zebrafish embryogenesis

Abundance and Diversity of Glycoconjugates Visualized Cytochemically in the Nervous System.

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