V-ATPase B1-subunit promoter drives expression of EGFP in intercalated cells of kidney, clear cells of epididymis and airway cells of lung in transgenic mice

Miller, R. Lance; Zhang, Ping; Smith, Maren L.; Beaulieu, Valerie; Păunescu, Teodor G.; Brown, Dennis; Breton, Sylvie; Nelson, Raoul D.

doi:10.1152/ajpcell.00084.2004

Cited by 102 publications

(125 citation statements)

References 46 publications

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“…11 The 640-kD V 1 subunit is composed of subunits A-H. Mammals have two B subunits, the ubiquitous B2 isoform and the B1 isoform, which is restricted to specialized epithelia of the inner ear, epididymis, and intercalated cells. 12 Numerous homozygous and compound heterozygous missense, nonsense, frameshift, and splice site mutations along the B1 subunit gene ATP6V1B1 have been reported in individuals with congenital dRTA. 3,13 We previously investigated disease-causing missense B1 subunit mutations in vitro.…”

Section: Urinary Acidification Is Achieved By Hmentioning

confidence: 99%

The Vacuolar H+-ATPase B1 Subunit Polymorphism p.E161K Associates with Impaired Urinary Acidification in Recurrent Stone Formers

Dhayat

Schaller

Albano

et al. 2015

JASN

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Mutations in the vacuolar-type H + -ATPase B1 subunit gene ATP6V1B1 cause autosomal-recessive distal renal tubular acidosis (dRTA). We previously identified a single-nucleotide polymorphism (SNP) in the human B1 subunit (c.481G.A; p.E161K) that causes greatly diminished pump function in vitro. To investigate the effect of this SNP on urinary acidification, we conducted a genotype-phenotype analysis of recurrent stone formers in the Dallas and Bern kidney stone registries. Of 555 patients examined, 32 (5.8%) were heterozygous for the p.E161K SNP, and the remaining 523 (94.2%) carried two wild-type alleles. After adjustment for sex, age, body mass index, and dietary acid and alkali intake, p.E161K SNP carriers had a nonsignificant tendency to higher urinary pH on a random diet (6.31 versus 6.09; P=0.09). Under an instructed low-Ca and low-Na diet, urinary pH was higher in p.E161K SNP carriers (6.56 versus 6.01; P,0.01). Kidney stones of p.E161K carriers were more likely to contain calcium phosphate than stones of wild-type patients. In acute NH 4 Cl loading, p.E161K carriers displayed a higher trough urinary pH (5.34 versus 4.89; P=0.01) than wild-type patients. Overall, 14.6% of wild-type patients and 52.4% of p.E161K carriers were unable to acidify their urine below pH 5.3 and thus, can be considered to have incomplete dRTA. In summary, our data indicate that recurrent stone formers with the vacuolar H + -ATPase B1 subunit p.E161K SNP exhibit a urinary acidification deficit with an increased prevalence of calcium phosphatecontaining kidney stones. The burden of E161K heterozygosity may be a forme fruste of dRTA.

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Section: Urinary Acidification Is Achieved By Hmentioning

confidence: 99%

The Vacuolar H+-ATPase B1 Subunit Polymorphism p.E161K Associates with Impaired Urinary Acidification in Recurrent Stone Formers

Dhayat

Schaller

Albano

et al. 2015

JASN

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“…NM_039350) has been successfully used to drive expression of both enhanced green fluorescent protein (EGFP) and the Cre-recombinase (Cre) into renal intercalated cells. 14,15 Importantly, preliminary experiments revealed that the promoter is likely to be insensitive to a high-salt diet (Supplemental Figure 1). We used this promoter fragment to drive the expression of human pendrin (hPDS/SLC26A4) cDNA in intercalated cells of the connecting tubule and the cortical collecting duct (CCD; detailed methods of the transgene construction and genotyping can be found in Supplemental Material and Supplemental Table 1).…”

Section: Generation Of a Mouse Model Overexpressing Pendrin In The Inmentioning

confidence: 99%

“…Figure 1C shows that high levels of the human pendrin transcript were detected by RT-PCR in the renal cortex and medulla of transgenic B1-hPDS (Tg B1-hPDS ) mice, whereas it was not present in the wild-type littermates. We previously reported that, beyond expression in renal intercalated cells, our ATP6V1B1 promoter fragment was able to drive expression of EGFP in epididymis, uterus, small and large intestines, and nonciliated airway epithelial cells 15 and Cre-recombinase in the brain. 14 Thus, we tested expression of the transgene in these different tissues ( Figure 1D).…”

Section: Generation Of a Mouse Model Overexpressing Pendrin In The Inmentioning

confidence: 99%

“…Ectopic expression of hPDS in a-intercalated cells was expected, because our B1 promoter fragment was shown to drive expression of EGFP and Cre in both intercalated cell subtypes. 14,15 Noteworthy, the expression of the transgene had no particular impact on AE1 or the V H + -ATPase cellular or subcellular localization.…”

Section: Generation Of a Mouse Model Overexpressing Pendrin In The Inmentioning

confidence: 99%

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Overexpression of Pendrin in Intercalated Cells Produces Chloride-Sensitive Hypertension

Jacques

Picard

Miller

et al. 2013

Journal of the American Society of Nephrology

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Inherited and acquired disorders that enhance the activity of transporters mediating renal tubular Na + reabsorption are well established causes of hypertension. It is unclear, however, whether primary activation of an Na + -independent chloride transporter in the kidney can also play a pathogenic role in this disease. Here, mice overexpressing the chloride transporter pendrin in intercalated cells of the distal nephron (Tg B1-hPDS mice) displayed increased renal absorption of chloride. Compared with normal mice, these transgenic mice exhibited a delayed increase in urinary NaCl and ultimately, developed hypertension when exposed to a high-salt diet. Administering the same sodium intake as NaHCO 3 instead of NaCl did not significantly alter BP, indicating that the hypertension in the transgenic mice was chloride-sensitive. Moreover, excessive chloride absorption by pendrin drove parallel absorption of sodium through the epithelial sodium channel ENaC and the sodium-driven chloride/bicarbonate exchanger (Ndcbe), despite an appropriate downregulation of these sodium transporters in response to the expanded vascular volume and hypertension. In summary, chloride transport in the distal nephron can play a primary role in driving NaCl transport in this part of the kidney, and a primary abnormality in renal chloride transport can provoke arterial hypertension. Thus, we conclude that the chloride/bicarbonate exchanger pendrin plays a major role in controlling net NaCl absorption, thereby influencing BP under conditions of high salt intake.

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“…Here the risk of contamination with other segments or cell populations is much higher. Transgenic mouse models expressing EGFP or other fluorescent proteins under the control of cell or segmentspecific promoters have become available over the last few years such as mice expressing EGFP in intercalated cells driven by the promoter for the B1 H + -ATPase subunit 27 . Kidneys from these mice can be used to isolate large quantitities of nephron segments or cells after digestion of the organ using fluorescence-guided sorting of segments or cells (COPAS: complex object parametric analyzer and sorter) 28 .…”

Section: Substructure Isolationmentioning

confidence: 99%

Toward Quantitative Proteomics of Organ Substructures: Implications for Renal Physiology

Velić

Maček

Wagner

2010

Seminars in Nephrology

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AcknowledgementsResearch in the laboratories of the authors has been supported by grants from the Minstry of Science, Baden-Wuerttenberg (to BM) and the Swiss National Science Foundation, the 6 th and 7 th EU Framework projects (EuReGene and EUNEFRON) (to CAW). We thank MatthiasMann for critically reading and discussing the manuscript. Summary 2Organs are complex structures that consist of multiple tissues with different levels of gene expression. To achieve a comprehensive coverage and accurate quantitation data, organs should ideally be separated into morphological and/or functional substructures prior to gene or protein expression analysis. However, due to complex morphology and elaborate isolation protocols, this was so far often difficult to achieve. Kidneys are organs where functional and morphological subdivision is especially important. Each subunit of the kidney, the nephron, itself consists of more than 10 subsegments with distinct morphological and functional characteristics. For a full understanding of kidney physiology, global gene and protein expression analyses have to be performed at the level of the nephron subsegments; however, such studies have so far been extremely rare.Here we describe the latest approaches in quantitative high accuracy mass spectrometrybased proteomics and their application to quantitative proteomics studies of the whole kidney and nephron subsegments, both in humans and in animal models. We compare these studies with similar studies performed on other organ substructures. We argue that the newest technologies used for preparation, processing and measurement of small amounts of starting material are finally enabling global and subsegment-specific quantitative measurement of protein levels in the kidney and other organs. These new technologies and approaches are making a decisive impact on our understanding of the (patho)physiological processes at the molecular level.3

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V-ATPase B1-subunit promoter drives expression of EGFP in intercalated cells of kidney, clear cells of epididymis and airway cells of lung in transgenic mice

Cited by 102 publications

References 46 publications

The Vacuolar H+-ATPase B1 Subunit Polymorphism p.E161K Associates with Impaired Urinary Acidification in Recurrent Stone Formers

The Vacuolar H+-ATPase B1 Subunit Polymorphism p.E161K Associates with Impaired Urinary Acidification in Recurrent Stone Formers

Overexpression of Pendrin in Intercalated Cells Produces Chloride-Sensitive Hypertension

Toward Quantitative Proteomics of Organ Substructures: Implications for Renal Physiology

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