Clinical and Genetic Spectrum of Bartter Syndrome Type 3

Seys, Elsa; Andrini, Olga; Keck, Mathilde; Mansour‐Hendili, Lamisse; Courand, Pierre‐Yves; Simian, Christophe; Deschenes, Georges; Kwon, Thérèsa; Bertholet‐Thomas, Aurélia; Bobrie, Guillaume; Borde, Jean Sébastien; Bourdat-Michel, Guylhène; Decramer, Stéphane; Cailliez, Mathilde; Krug, Pauline; Cozette, P; Delbet, Jean Daniel; Dubourg, Laurence; Chaveau, Dominique; Fila, Marc; Jourde-Chiche, Noémie; Knebelmann, Bertrand; Lavocat, Marie-Pierre; Lemoine, Sandrine; Djeddi, D.; Llanas, Brigitte; Louillet, Férielle; Mérieau, Elodie; Mileva, Maria; Mota-Vieira, Luísa; Mousson, Christiane; Nobili, François; Novo, Robert; Roussey-Kesler, Gwénaëlle; Vrillon, Isabelle; Walsh, Stephen B.; Teulon, Jacques; Blanchard, Anne; Vargas‐Poussou, Rosa

doi:10.1681/asn.2016101057

Cited by 98 publications

(141 citation statements)

References 44 publications

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“…Shao et al reported that deletion of the complete CLCNKB gene was the most common variant in Chinese patients with cBS, and the frequency of whole gene deletion was up to 9/28 (32%). Patients who carried the whole CLCNKB gene deletion variant showed an early-onset, severe phenotype with greater urinary salt wasting (Han et al, 2017;Seys et al, 2017;Li et al, 2019). Taken together, our results support that the whole CLCNKB gene deletion may account for a more severe phenotype of patients.…”

Section: [239g > A]; C[1053-1g > A] and C[239g > A];supporting

confidence: 76%

Splicing Characterization of CLCNKB Variants in Four Patients With Type III Bartter Syndrome

et al. 2020

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Section: [239g > A]; C[1053-1g > A] and C[239g > A];supporting

confidence: 76%

Splicing Characterization of CLCNKB Variants in Four Patients With Type III Bartter Syndrome

et al. 2020

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“…The disease may have features of BS (either antenatal or classic) and/or Gitelman syndrome. 66 ClC-K2 deficient mice exhibit salt losing phenotype, with compensatory increased RAAS axis, hypotension, and increased prostaglandin E2 generation; interestingly, the mice show a blunted response to both furosemide and thiazides, indicating a combined defective salt absorption along both TAL and DT. 67 Activating mutations of the CaSR have been associated with hypocalcemia and hypercalciuria, and sometime hypomagnesemia.…”

Section: Bartter Syndrome (Bs)mentioning

confidence: 98%

The importance of the thick ascending limb of Henle’s loop in renal physiology and pathophysiology

Zacchia

Capolongo

Rinaldi

et al. 2018

IJNRD

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The thick ascending limb (TAL) of Henle’s loop is a crucial segment for many tasks of the nephron. Indeed, the TAL is not only a mainstay for reabsorption of sodium (Na+), potassium (K+), and divalent cations such as calcium (Ca2+) and magnesium (Mg2+) from the luminal fluid, but also has an important role in urine concentration, overall acid–base homeostasis, and ammonia cycle. Transcellular Na+ transport along the TAL is a prerequisite for Na+, K+, Ca2+, Mg2+ homeostasis, and water reabsorption, the latter through its contribution in the generation of the cortico-medullar osmotic gradient. The role of this nephron site in acid–base balance, via bicarbonate reabsorption and acid secretion, is sometimes misunderstood by clinicians. This review describes in detail these functions, reporting in addition to the well-known molecular mechanisms, some novel findings from the current literature; moreover, the pathophysiology and the clinical relevance of primary or acquired conditions caused by TAL dysfunction are discussed. Knowing the physiology of the TAL is fundamental for clinicians, for a better understanding and management of rare and common conditions, such as tubulopathies, hypertension, and loop diuretics abuse.

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“…Ca 2+ increases the open probability of ClC‐K channels (Gradogna, Babini, Picollo, & Pusch, ; Gradogna, Fenollar‐Ferrer, Forrest, & Pusch, ) by acting on two amino acids (i.e., E261 and D278). In this study, we got interested in two pathological mutations (Seys et al, ) located in close vicinity to the calcium‐binding site (Gradogna et al, ; Gradogna et al, ): A254V (α helix I; c.761C>T, p.Ala254Val) and G465R (α helix O; c.1393G>A, p.Gly465Arg; see Figure b for localization).…”

Section: Introductionmentioning

confidence: 99%

“…A relatively large number of pathological CLCNKB mutations positioned throughout the whole length of the protein and affecting particularly the pore and dimer interface has been identified (Andrini et al, 2014;Brochard et al, 2009;Keck et al, 2013;Konrad et al, 2000;Lee et al, 2012;Seys et al, 2017;Stolting, Bungert-Plumke, Franzen, & Fahlke, 2015;Yu et al, 2009;see Andrini et al, 2015 for review). Functional studies began to assess the currents generated by several mutants in Xenopus laevis oocytes immediately after the discovery of Barttin (Estevez et al, 2001;Waldegger et al, 2002), an effort that was continued by attempts to describe the functional consequences of CLCNKB mutations (Andrini et al, 2014;Andrini et al, 2015;Cheng, Lo, Chen, Huang, & Lin, 2017;Martinez & Maduke, 2008;Stolting et al, 2015;Yu et al, 2009).…”

mentioning

confidence: 99%

“…We focused our efforts on the functional characterization of five pathological CLCNKB mutations at the dimer interface: A204T (c.610G>A, p.Ala204Thr; Garcia Castano et al, 2013;Rodriguez-Soriano, Vallo, Perez de Nanclares, Bilbao, & Castano, 2005;Simon et al, 1997); A210V (c.629C>T, p.Ala210Val; Yu et al, 2009); P216L (c.647C>T, p.Pro216Leu; Lee et al, 2012;S218N (c.653G>A, p.Ser218Asn;Seys et al, 2017); and G219C (c.655G>T, p.Gly219Cys; Seys et al, 2017; see Figure 6b for localization). A second region important for gating and ion selectivity, around α helix N (Dutzler, Campbell, & MacKinnon, 2003;Dutzler et al, 2002) comprised mutations G424R (c.1270G>A, p.Gly424Arg;Seys et al, 2017) and G437R (c.1309G>C, p.Gly437Arg; Lee et al, 2012;see Figure 6 for localization). Mutations in α helix N encountered in ClC-5 (Lourdel et al, 2012) and in ClC-1 (Pusch, 2002) cause modifications in conductance and gating or alter expression.…”

mentioning

confidence: 99%

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Analysis ofCLCNKBmutations at dimer‐interface, calcium‐binding site, and pore reveals a variety of functional alterations in ClC‐Kb channel leading to Bartter syndrome

et al. 2019

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Pathological missense mutations in CLCNKB gene give a wide spectrum of clinical phenotypes in Bartter syndrome type III patients. Molecular analysis of the mutated ClC‐Kb channels can be helpful to classify the mutations according to their functional alteration. We investigated the functional consequences of nine mutations in the CLCNKB gene causing Bartter syndrome. We first established that all tested mutations lead to decreased ClC‐Kb currents. Combining electrophysiological and biochemical methods in Xenopus laevis oocytes and in MDCKII cells, we identified three classes of mutations. One class is characterized by altered channel trafficking. p.A210V, p.P216L, p.G424R, and p.G437R are totally or partially retained in the endoplasmic reticulum. p.S218N is characterized by reduced channel insertion at the plasma membrane and altered pH‐sensitivity; thus, it falls in the second class of mutations. Finally, we found a novel class of functionally inactivated mutants normally present at the plasma membrane. Indeed, we found that p.A204T alters the pH‐sensitivity, p.A254V abolishes the calcium‐sensitivity. p.G219C and p.G465R are probably partially inactive at the plasma membrane. In conclusion, most pathogenic mutants accumulate partly or totally in intracellular compartments, but some mutants are normally present at the membrane surface and simultaneously show a large range of altered channel gating properties.

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Clinical and Genetic Spectrum of Bartter Syndrome Type 3

Cited by 98 publications

References 44 publications

Splicing Characterization of CLCNKB Variants in Four Patients With Type III Bartter Syndrome

Splicing Characterization of CLCNKB Variants in Four Patients With Type III Bartter Syndrome

The importance of the thick ascending limb of Henle’s loop in renal physiology and pathophysiology

Analysis ofCLCNKBmutations at dimer‐interface, calcium‐binding site, and pore reveals a variety of functional alterations in ClC‐Kb channel leading to Bartter syndrome

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Clinical and Genetic Spectrum of Bartter Syndrome Type 3

Cited by 98 publications

References 44 publications

Splicing Characterization of CLCNKB Variants in Four Patients With Type III Bartter Syndrome

Splicing Characterization of CLCNKB Variants in Four Patients With Type III Bartter Syndrome

The importance of the thick ascending limb of Henle&rsquo;s loop in renal physiology and pathophysiology

Analysis ofCLCNKBmutations at dimer‐interface, calcium‐binding site, and pore reveals a variety of functional alterations in ClC‐Kb channel leading to Bartter syndrome

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The importance of the thick ascending limb of Henle’s loop in renal physiology and pathophysiology