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Showing content from http://www.ncbi.nlm.nih.gov/pubmed/19185582 below:

Tissue-specific amino acid transporter partners ACE2 and collectrin differentially interact with hartnup mutations

Affiliations

• ¹ Institute of Physiology and Zürich Center for Integrative Human Physiology, University of Zurich, Zurich, Switzerland.

• PMID: 19185582
• PMCID: PMC7094282
• DOI: 10.1053/j.gastro.2008.10.055

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Simone M R Camargo et al. Gastroenterology. 2009 Mar.

• ¹ Institute of Physiology and Zürich Center for Integrative Human Physiology, University of Zurich, Zurich, Switzerland.

• PMID: 19185582
• PMCID: PMC7094282
• DOI: 10.1053/j.gastro.2008.10.055

Item in Clipboard

Background & aims: Hartnup amino acid transporter B(0)AT1 (SLC6A19) is the major luminal sodium-dependent neutral amino acid transporter of small intestine and kidney proximal tubule. The expression of B(0)AT1 in kidney was recently shown to depend on its association with collectrin (Tmem27), a protein homologous to the membrane-anchoring domain of angiotensin-converting enzyme (ACE) 2.

Methods: Because collectrin is almost absent from small intestine, we tested the hypothesis that it is ACE2 that interacts with B(0)AT1 in enterocytes. Furthermore, because B(0)AT1 expression depends on an associated protein, we tested the hypothesis that Hartnup-causing B(0)AT1 mutations differentially impact on B(0)AT1 interaction with intestinal and kidney accessory proteins.

Results: Immunofluorescence, coimmunoprecipitation, and functional experiments using wild-type and ace2-null mice showed that expression of B(0)AT1 in small intestine critically depends on ACE2. Coexpressing new and previously identified Hartnup disorder-causing missense mutations of B(0)AT1 with either collectrin or ACE2 in Xenopus laevis oocytes showed that the high-frequency D173N and the newly identified P265L mutant B(0)AT1 transporters can still be activated by ACE2 but not collectrin coexpression. In contrast, the human A69T and R240Q B(0)AT1 mutants cannot be activated by either of the associated proteins, although they function as wild-type B(0)AT1 when expressed alone.

Conclusions: We thus show that ACE2 is necessary for the expression of the Hartnup transporter in intestine and suggest that the differential functional association of mutant B(0)AT1 transporters with ACE2 and collectrin in intestine and kidney, respectively, participates in the phenotypic heterogeneity of human Hartnup disorder.

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ACE2 and B ⁰ AT1…

ACE2 and B ⁰ AT1 colocalization and functional interaction. ( A ) Immunofluorescence…

ACE2 and B⁰AT1 colocalization and functional interaction. (A) Immunofluorescence analysis shows that B⁰AT1 protein expression is lost in small intestine of ace2-null mice. Small intestine sections from ace2^+/y and ace2^−/y were colabeled with antibodies against ACE2 (green) and B⁰AT1 (red) and additionally viewed by phase contrast (PC). (B) Western blot analysis shows that B⁰AT1 is absent in small intestine but present in kidney brush border membranes of ace2-null mice, whereas B⁰AT1 is expressed in small intestine and absent from kidney brush border membranes in collectrin-null mice. The loading of brush border membranes (2.5–20 μg) was tested using a β-actin antibody (βA). Note that male ace2^+/y or ace2^−/y and female ace2^+/+ or ace2^−/− mice were used with similar results. (C) Coimmunoprecipitation shows interaction of ACE2 with B⁰AT1 in mouse small intestine. Complexes were immunoprecipitated (IP) from small intestine brush border membrane vesicles (BBMVs) using anti-B⁰AT1 antibody (AB) and analyzed by Western blot (WB) using anti-mouse ACE2 antibody. (D) Na⁺-dependent uptake of l -isoleucine (L-Ile) is abolished in ileum segments from ace2^−/y mice. The transport was measured in the presence (white bar) and in the absence (black bar) of sodium. Data points represent mean values of 4 intestinal ring uptakes from independent experiments ± SEM, ***P < .001. ns, not significant.

Differential function of Hartnup mutations…

Differential function of Hartnup mutations coexpressed with collectrin or ACE2 in X laevis…

Differential function of Hartnup mutations coexpressed with collectrin or ACE2 in X laevis oocytes. Wild-type and mutant human B⁰AT1 are shown in this figure as 3 groups with different functional characteristics and labeled A–C. (A) The transport function and the surface expression of both wild-type and nonsynonymous SNP V252I of B⁰AT1 are increased by coexpression with human collectrin or mouse ACE2. (B) The relatively low transport activity of B⁰AT1 D173N and P265L mutants expressed alone is increased by coexpression with ACE2 but not with collectrin. The surface expression of the D173N mutant is also significantly increased by coexpression with ACE2. (C) The wild-type–like function of the A69T or R240Q mutants expressed alone is not increased in the presence of collectrin or ACE2, although in the case of A69T its surface expression is increased. The upper panels of A–C show the transport function measured as radiolabeled l -isoleucine (L-Ile) uptake (means ± SEM of 13–31 oocytes from 3 independent experiments), and the middle panel shows the transport function as current measured by TEVC (9–11 oocytes from 3 batches). *P < .05, ***P < .001. The lower panels show the surface expression assayed by Western blot using surface-biotinylated proteins and a representative Western blot. The data correspond to the means ± SEM (n = 3–5 independent experiments) of the results normalized to the value obtained for B⁰AT1 expressed alone. For the transport experiments, the significance was evaluated using analysis of variance with Tukey posttest and for the surface biotinylation the comparison of means was performed by unpaired t test. (D) B⁰AT1 and the mutants D173N, P265L, R240Q, and A69T interact with ACE2 in X laevis oocytes. The transporters expressed alone or together with human ACE2 were immunoprecipitated (IP) from oocyte lysates using anti-human B⁰AT1 antibody and complexes were analyzed by Western blot (WB) using anti-human ACE2 antibody. NI, noninjected.

The ion dependency of D173N,…

The ion dependency of D173N, P265L, A69T, and R240Q coexpressed with ACE2 or…

The ion dependency of D173N, P265L, A69T, and R240Q coexpressed with ACE2 or collectrin is not altered; transport is Na⁺ but not Cl⁻ dependent. Wild-type human B⁰AT1 (WT) and the mutants D173N, P265L, A69T, and R240Q were expressed alone or with human collectrin or mouse ACE2. The ion dependence was tested by substituting Na⁺ with N-methyl- d -glucamine (NMDG) and substituting Cl⁻ with gluconate. Function was assayed by influx of radiolabeled l -isoleucine (L-Ile). For each mutation, 3 independent experiments (15–24 oocytes) were pooled. Comparison of means was performed by analysis of variance with Tukey as posttest. Data represent means ± SEM. *P < .05, **P < .01, ***P < .001. ns, not significant.

The B ⁰ AT1 mutants…

The B ⁰ AT1 mutants R57C, G93R, L242P, E501K, and P579L exhibit no…

The B⁰AT1 mutants R57C, G93R, L242P, E501K, and P579L exhibit no transport activity when expressed alone or coexpressed with collectrin or ACE2. Function was assayed by influx of radiolabeled l -isoleucine (L-Ile) (upper panels) or TEVC (middle panels). For each mutant, 3 independent experiments (13–31 oocytes for influx and 9–11 for TEVC) were pooled. Comparison of means was performed by analysis of variance with Tukey as posttest. Data represent means ± SEM. ns, not significant. Cell surface expression of labeled proteins (lower panels) was analyzed by Western blot. The bands were quantified and data normalized to the values obtained from oocytes expressing B⁰AT1 proteins alone. For each mutation, 3 to 4 independent experiments were pooled. Comparison of means was performed by unpaired t test. Data represent means ± SEM. *P < .05. ns, not significant.

Missense mutations in the SLC6A19…

Missense mutations in the SLC6A19 gene causing Hartnup disorder. The model of B…

Missense mutations in the SLC6A19 gene causing Hartnup disorder. The model of B⁰AT1 is based on the Slc6 bacterial homologue from Aquifex aeolicus LeuT_Aa and the transmembrane segments are numbered. The localization of mutations causing a loss of surface expression (R57, G93, L242, E501, P579) is depicted in the left panel. The sites of mutations leading to a differential interaction with the 2 accessory proteins (D173 and P265) are depicted as black spheres on the middle panel, and the sites of the mutations preventing both accessory proteins of stimulating the transport function are depicted on the right panel (A69 and R240).

Function of human B…

Function of human B ⁰ AT1 coexpressed with orthologues of collectrin and…

Function of human B⁰AT1 coexpressed with orthologues of collectrin and ACE2 in X laevis oocytes. (A) Coexpression of ACE2 or human collectrin increases B⁰AT1 function in X laevis oocytes. Tracer flux experiments (upper graph, n = 16–32) and TEVC (lower graph, n = 11) show that human B⁰AT1 (hB⁰AT1) coexpressed with human ACE2 (hACE2), mouse ACE2 (mACE2), or human collectrin (hColl) transports l -isoleucine more efficiently than when expressed alone or in combination with mouse collectrin (mColl). Data points represent means ± SEM. ***P < .001. ns, not significant. (B) Human B⁰AT1 function is increased by coexpressed human ACE2 independent of its protease activity. The protease-dead human ACE2 mutant (ACE2 R273Q) stimulated the human B⁰AT1-mediated l -isoleucine influx to the same extent as wild-type human ACE2. Data points represent means ± SEM (n = 15–16). ns, not significant.

Functional characterization of the…

Functional characterization of the complex formed by human B ⁰ AT1 and…

Functional characterization of the complex formed by human B⁰AT1 and ACE2 in X laevis oocytes. (A) The amino acid transport by human B⁰AT1 coexpressed with mouse ACE2 in X laevis oocytes is Na⁺ but not Cl⁻ dependent. The ion dependence was tested by substituting Na⁺ by N-methyl- d -glucamine (NMDG) or Li⁺ and Cl⁻ by gluconate in the superfusion solution used for TEVC. The values were normalized to the current obtained by superfusion of the oocytes with 10 mmol/L l -isoleucine in solution containing Na⁺ and Cl⁻ (I_norm). Comparison of means was performed by analysis of variance with Tukey as posttest. Each data point represents the mean ± SEM (n = 16). ***P < .001. (B) Amino acid transport by human B⁰AT1 coexpressed with mouse ACE2 in X laevis oocytes is maximal at neutral pH. The pH dependence of the transport was measured by TEVC in oocytes clamped at –50 mV and superfused with Na⁺ solution buffered at pH 5.5, 6.5, 7.4, or 8.0. Values were normalized to the current obtained by superfusion of oocytes with 10 mmol/L l -isoleucine in solution pH 7.4 (I_norm). Comparison of means was performed by analysis of variance with Tukey as posttest. Each data point represents the mean ± SEM (n = 9). *P < .05, **P < .01. (C–E) Human B⁰AT1 coexpressed with ACE2 transports a broad range of neutral amino acids with low affinity. (C) The substrate selectivity of human B⁰AT1 coexpressed with mouse ACE2 was measured by TEVC in oocytes clamped at –50 mV and superfused with Na⁺ solution containing 1 mmol/L (white bars) or 10 mmol/L (black bars) of amino acids. The currents induced by the amino acids were normalized to the currents obtained in oocytes perfused with 10 mmol/L l -isoleucine (I_norm). Data are shown as mean values ± SEM (n = 8–11) and the amino acids are indicated in single letter code. (D and E) The K_0.5 and V_max for l -isoleucine and Na⁺ of human B⁰AT1 coexpressed with mouse ACE2 was estimated using TEVC. For the Na⁺ concentration dependence experiments, the cells were first equilibrated with the indicated Na⁺ concentration (0, 1, 5, 10, 30, 50, 70, and 100 mmol/L) before the perfusate containing l -isoleucine (10 mmol/L) was applied. For the l -isoleucine concentration dependence experiments, the cells were perfused with increasing concentrations of l -isoleucine (0.1, 0.3, 1, 3, and 10 mmol/L). The continuous line is the nonlinear regression fit of the Michaelis–Menten equation to the data. Each data point represents the mean ± SEM (C, n = 26–27; D, n = 10–22).

Pedigrees of 4 families…

Pedigrees of 4 families with new Hartnup disorder mutations. ( A )…

Pedigrees of 4 families with new Hartnup disorder mutations. (A) Danish pedigree: 2 of 3 siblings were compound heterozygous for P265L and L242P. The symptoms observed were quite diverse between the 2 sisters. The younger one was diagnosed with Hartnup disorder in early childhood due to pellagra-like skin rash and an atactic gait that improved with administration of niacin. The older affected sibling never showed skin pathologies or ataxia. (B) Another Danish pedigree, where the only child affected was a compound heterozygous for A69T and the original Hartnup mutation IVS8+2T→G. This patient was the first child of unrelated parents and was diagnosed at 1 year of age after a suspected seizure prompted a metabolic screening of urine. Plasma amino acids and electroencephalography were normal. The patient subsequently had normal growth and development without epilepsy, ataxia, or pellagra. (C) The other Danish patient was a compound heterozygous for P579L and the original Hartnup mutation IVS8+2T→G. This patient was the second child of unrelated parents and was diagnosed at 2 years of age after onset of partial complex epilepsy with great difficulty to control seizures. The patient had normal plasma amino acids and never had ataxia or pellagra. (D) Another patient from a German family was diagnosed as homozygous for the new missense mutation G93R. This patient was diagnosed at 6 years of age during a migraine workup and also never had ataxia or pellagra. The affected subjects are depicted as filled symbols.

• A protein complex in the brush-border membrane explains a Hartnup disorder allele.

  Kowalczuk S, Bröer A, Tietze N, Vanslambrouck JM, Rasko JE, Bröer S. Kowalczuk S, et al. FASEB J. 2008 Aug;22(8):2880-7. doi: 10.1096/fj.08-107300. Epub 2008 Apr 18. FASEB J. 2008. PMID: 18424768

• Human intestine luminal ACE2 and amino acid transporter expression increased by ACE-inhibitors.

  Vuille-dit-Bille RN, Camargo SM, Emmenegger L, Sasse T, Kummer E, Jando J, Hamie QM, Meier CF, Hunziker S, Forras-Kaufmann Z, Kuyumcu S, Fox M, Schwizer W, Fried M, Lindenmeyer M, Götze O, Verrey F. Vuille-dit-Bille RN, et al. Amino Acids. 2015 Apr;47(4):693-705. doi: 10.1007/s00726-014-1889-6. Epub 2014 Dec 23. Amino Acids. 2015. PMID: 25534429

• Collectrin and ACE2 in renal and intestinal amino acid transport.

  Singer D, Camargo SM. Singer D, et al. Channels (Austin). 2011 Sep-Oct;5(5):410-23. doi: 10.4161/chan.5.5.16470. Epub 2011 Sep 1. Channels (Austin). 2011. PMID: 21814048 Review.

• Orphan transporter SLC6A18 is renal neutral amino acid transporter B0AT3.

  Singer D, Camargo SM, Huggel K, Romeo E, Danilczyk U, Kuba K, Chesnov S, Caron MG, Penninger JM, Verrey F. Singer D, et al. J Biol Chem. 2009 Jul 24;284(30):19953-60. doi: 10.1074/jbc.M109.011171. Epub 2009 May 28. J Biol Chem. 2009. PMID: 19478081 Free PMC article.

• The role of the neutral amino acid transporter B0AT1 (SLC6A19) in Hartnup disorder and protein nutrition.

  Bröer S. Bröer S. IUBMB Life. 2009 Jun;61(6):591-9. doi: 10.1002/iub.210. IUBMB Life. 2009. PMID: 19472175 Free PMC article. Review.

• SARS-CoV-2 receptor ACE2 gene expression in small intestine correlates with age.

  Vuille-Dit-Bille RN, Liechty KW, Verrey F, Guglielmetti LC. Vuille-Dit-Bille RN, et al. Amino Acids. 2020 Jul;52(6-7):1063-1065. doi: 10.1007/s00726-020-02870-z. Epub 2020 Jul 5. Amino Acids. 2020. PMID: 32627059 Free PMC article.

• SARS-CoV-2 first contact: Spike-ACE2 interactions in COVID-19.

  Nesci S. Nesci S. Chem Biol Drug Des. 2021 Aug;98(2):207-211. doi: 10.1111/cbdd.13898. Epub 2021 Jun 21. Chem Biol Drug Des. 2021. PMID: 34047452 Free PMC article.

• Unpuzzling COVID-19: tissue-related signaling pathways associated with SARS-CoV-2 infection and transmission.

  Battagello DS, Dragunas G, Klein MO, Ayub ALP, Velloso FJ, Correa RG. Battagello DS, et al. Clin Sci (Lond). 2020 Aug 28;134(16):2137-2160. doi: 10.1042/CS20200904. Clin Sci (Lond). 2020. PMID: 32820801 Free PMC article.

• Decoding the bidirectional relationship between gut microbiota and COVID-19.

  Ralli T, Saifi Z, Rathee A, Aeri V, Kohli K. Ralli T, et al. Heliyon. 2023 Mar;9(3):e13801. doi: 10.1016/j.heliyon.2023.e13801. Epub 2023 Feb 17. Heliyon. 2023. PMID: 36811017 Free PMC article. Review.

• Angiotensin-converting enzyme 2 deficiency accelerates and angiotensin 1-7 restores age-related muscle weakness in mice.

  Takeshita H, Yamamoto K, Nozato S, Takeda M, Fukada SI, Inagaki T, Tsuchimochi H, Shirai M, Nozato Y, Fujimoto T, Imaizumi Y, Yokoyama S, Nagasawa M, Hamano G, Hongyo K, Kawai T, Hanasaki-Yamamoto H, Takeda S, Takahashi T, Akasaka H, Itoh N, Takami Y, Takeya Y, Sugimoto K, Nakagami H, Rakugi H. Takeshita H, et al. J Cachexia Sarcopenia Muscle. 2018 Oct;9(5):975-986. doi: 10.1002/jcsm.12334. Epub 2018 Sep 11. J Cachexia Sarcopenia Muscle. 2018. PMID: 30207087 Free PMC article.

1. 1. Kleta R., Romeo E., Ristic Z. Mutations in SLC6A19, encoding B0AT1, cause Hartnup disorder. Nat Genet. 2004;36:999–1002. - PubMed
2. 1. Seow H.F., Broer S., Broer A. Hartnup disorder is caused by mutations in the gene encoding the neutral amino acid transporter SLC6A19. Nat Genet. 2004;36:1003–1007. - PubMed
3. 1. Danilczyk U., Sarao R., Remy C. Essential role for collectrin in renal amino acid transport. Nature. 2006;444:1088–1091. - PubMed
4. 1. Malakauskas S.M., Quan H., Fields T.A. Aminoaciduria and altered renal expression of luminal amino acid transporters in mice lacking novel gene collectrin. Am J Physiol Renal Physiol. 2007;292:F533–F544. - PubMed
5. 1. Crackower M.A., Sarao R., Oudit G.Y. Angiotensin-converting enzyme 2 is an essential regulator of heart function. Nature. 2002;417:822–828. - PubMed

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