A sequence upstream of canonical PDZ-binding motif within CFTR COOH-terminus enhances NHERF1 interaction

Sharma, Neeraj; LaRusch, Jessica; Sosnay, Patrick R.; Gottschalk, Laura; Lopez, Andrea; Pellicore, Matthew J.; Evans, Taylor A.; Davis, Emily; Atalar, Melis; Na, Chan Hyun; Rosson, Gedge D.; Belchis, Deborah A.; Milewski, Michał; Pandey, Akhilesh; Cutting, Garry R.

doi:10.1152/ajplung.00363.2016

Cited by 12 publications

(11 citation statements)

References 79 publications

(78 reference statements)

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“…In contrast, variants located more 3’ including nonsense (E1418X), and two frameshifts (E1418Rfs14X and S1435Gfs14X) that truncate protein at residue 1442 and 1459 respectively generated minimal to moderate amounts of mature truncated protein. The final two variants S1455X and Q1476X, showed no apparent effect on the steady-state amounts of the immature or mature truncated forms of CFTR when compared with WT, as shown previously ( Fig 1C, S2 Fig) [40, 41]. The nonsense and frameshift variants in the 3’region fell into three groups (A-C) based on effects on RNA and protein levels ( Fig 1D ).…”

Section: Resultssupporting

confidence: 78%

Capitalizing on the heterogeneous effects of CFTR nonsense and frameshift variants to inform therapeutic strategy for cystic fibrosis

et al. 2018

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CFTR modulators have revolutionized the treatment of individuals with cystic fibrosis (CF) by improving the function of existing protein. Unfortunately, almost half of the disease-causing variants in CFTR are predicted to introduce premature termination codons (PTC) thereby causing absence of full-length CFTR protein. We hypothesized that a subset of nonsense and frameshift variants in CFTR allow expression of truncated protein that might respond to FDA-approved CFTR modulators. To address this concept, we selected 26 PTC-generating variants from four regions of CFTR and determined their consequences on CFTR mRNA, protein and function using intron-containing minigenes expressed in 3 cell lines (HEK293, MDCK and CFBE41o-) and patient-derived conditionally reprogrammed primary nasal epithelial cells. The PTC-generating variants fell into five groups based on RNA and protein effects. Group A (reduced mRNA, immature (core glycosylated) protein, function <1% (n = 5)) and Group B (normal mRNA, immature protein, function <1% (n = 10)) variants were unresponsive to modulator treatment. However, Group C (normal mRNA, mature (fully glycosylated) protein, function >1% (n = 5)), Group D (reduced mRNA, mature protein, function >1% (n = 5)) and Group E (aberrant RNA splicing, mature protein, function > 1% (n = 1)) variants responded to modulators. Increasing mRNA level by inhibition of NMD led to a significant amplification of modulator effect upon a Group D variant while response of a Group A variant was unaltered. Our work shows that PTC-generating variants should not be generalized as genetic ‘nulls’ as some may allow generation of protein that can be targeted to achieve clinical benefit.

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Section: Resultssupporting

confidence: 78%

Capitalizing on the heterogeneous effects of CFTR nonsense and frameshift variants to inform therapeutic strategy for cystic fibrosis

et al. 2018

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“…25 cm ϫ 15 cm skin was collected from the abdominal region of a single donor. Eccrine sweat glands were dissected out from the skin dermis as previously described (12)(13)(14). Approximately 250 eccrine sweat glands were collected and pooled.…”

Section: Methodsmentioning

confidence: 99%

Integrated Transcriptomic and Proteomic Analysis of Human Eccrine Sweat Glands Identifies Missing and Novel Proteins

Na¹,

Sharma

Madugundu³

et al. 2019

Molecular & Cellular Proteomics

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This study reports the first indepth RNA and protein expression profiles of human sweat glands. RNA-sequencing and proteomic analysis were performed on ϳ250 sweat glands collected from a healthy individual. Data revealed ϳ13,300 protein-coding genes, ϳ53,400 non-coding genes, and ϳ6,100 proteins are expressed in eccrine sweat glands. Also, two missing and five novel proteins were identified. Integrated transcriptome and protein expression profile of eccrine sweat gland can be used to study the etiology of many diseases relevant to the sweat gland.

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“…To improve the model system, we then applied the differential display method to find differences in the genes expressed by CFDE cells (CF cells) and their CFTR-corrected counterparts, the latter also treated or not with CFTR inhibitors. The use of the CFTR inhibitor NPPB in the CFTR corrected CFDE cells (called CFDE/6Rep-CFTR cells) allowed us to identify functional differences due only to the Cl − transport activity of the CFTR -we selected the differential display spots in which the signal reverted to control values in the presence of NPPB -avoiding possible off-target effects of wild-type CFTR-transfected cells or effects exclusively due to the presence of the CFTR on the plasma membrane, as seems to be the case for regulated upon activation, normally T-expressed, and presumably secreted (RANTES) (Estell et al, 2003) and other PDZ (postsynaptic density protein 95/discs large/zona occludens protein-1 homologous)-dependent genes (Boucherot, Schreiber & Kunzelmann, 2001;Sharma et al, 2016;Watson et al, 2016). In this way, we found and characterized several CFTR-dependent genes, including c-Src (Gonzalez-Guerrico et al, 2002), mitochondrially encoded NADH:ubiquinone oxidoreductase core subunit 4 (MTND4) (Valdivieso et al, 2007) and CDGSH iron sulfur domain 1 (CISD1) (Taminelli et al, 2008).…”

Section: − As a Signalling Effector For Cftrmentioning

confidence: 99%

The chloride anion as a signalling effector

Valdivieso

Santa‐Coloma

2019

Biological Reviews

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The specific role of the chloride anion (Cl−) as a signalling effector or second messenger has been increasingly recognized in recent years. It could represent a key factor in the regulation of cellular homeostasis. Changes in intracellular Cl− concentration affect diverse cellular functions such as gene and protein expression and activities, post‐translational modifications of proteins, cellular volume, cell cycle, cell proliferation and differentiation, membrane potential, reactive oxygen species levels, and intracellular/extracellular pH. Cl− also modulates functions in different organelles, including endosomes, phagosomes, lysosomes, endoplasmic reticulum, and mitochondria. A better knowledge of Cl− signalling could help in understanding the molecular and metabolic changes seen in pathologies with altered Cl− transport or under physiological conditions. Here we review relevant evidence supporting the role of Cl− as a signalling effector.

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A sequence upstream of canonical PDZ-binding motif within CFTR COOH-terminus enhances NHERF1 interaction

Cited by 12 publications

References 79 publications

Capitalizing on the heterogeneous effects of CFTR nonsense and frameshift variants to inform therapeutic strategy for cystic fibrosis

Capitalizing on the heterogeneous effects of CFTR nonsense and frameshift variants to inform therapeutic strategy for cystic fibrosis

Integrated Transcriptomic and Proteomic Analysis of Human Eccrine Sweat Glands Identifies Missing and Novel Proteins

The chloride anion as a signalling effector

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