Cystic Fibrosis F508del Patients Have Apically Localized CFTR in a Reduced Number of Airway Cells

Penque, Deborah; Mendes, Filipa; Beck, Sebastian; Farinha, Carlos M.; Pacheco, Paula; Nogueira, Paulo; Lavinha, João; Malhó, Rui; Amaral, Margarida D.

doi:10.1038/labinvest.3780090

Cited by 89 publications

(107 citation statements)

References 67 publications

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“…CFTR protein, as detected by immunolocalization, was first reported in a few unidentified columnar cells within the superficial epithelium (Engelhardt et al, 1992(Engelhardt et al, , 1994 and more recently in a restricted population of columnar cells (Penque et al, 2000;Carvalho-Oliveira et al, 2004). We identified the ciliated cell as the only cell type expressing CFTR in nasal, bronchial, and proximal bronchiolar surface epithelia by high resolution LCM and coimmunostaining with antibodies against cellular markers (e.g., tubulin).…”

Section: Discussionmentioning

confidence: 95%

“…(Engelhardt et al, 1992(Engelhardt et al, , 1194Puchelle et al, 1992;Kalin et al, 1999;Penque et al, 2000). With the availability of very sensitive anti-CFTR mAbs (Mall et al, 2004) and LCM technologies, we initiated a comprehensive study to explore two major issues controversial in CF research: 1) the cell type specific localization of CFTR in the normal lung; and 2) the localization of ⌬F508 CFTR in native airway epithelium.…”

Section: Discussionmentioning

confidence: 99%

“…There are several possible reasons why our data and conclusions differ from some previous reports. First, our mAbs exhibit very high affinity for CFTR and hence may be less cross-reactive with other apical PM proteins in the CF lung compared with CFTR antibodies (Claass et al, 2000) used in previous studies (Kalin et al, 1999;Penque et al, 2000;Carvalho-Oliveira et al, 2004). Second, we applied multiple, complementary techniques to the same specimens.…”

Section: Expression Of ⌬F508 Cftr In Cf Airway Epitheliamentioning

confidence: 99%

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Characterization of Wild-Type and ΔF508 Cystic Fibrosis Transmembrane Regulator in Human Respiratory Epithelia

Kreda

Mall

Mengos

et al. 2005

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Previous studies in native tissues have produced conflicting data on the localization and metabolic fate of WT and ⌬F508 cystic fibrosis transmembrane regulator (CFTR) in the lung. Combining immunocytochemical and biochemical studies utilizing new high-affinity CFTR mAbs with ion transport assays, we examined both 1) the cell type and region specific expression of CFTR in normal airways and 2) the metabolic fate of ⌬F508 CFTR and associated ERM proteins in the cystic fibrosis lung. Studies of lungs from a large number of normal subjects revealed that WT CFTR protein localized to the apical membrane of ciliated cells within the superficial epithelium and gland ducts. In contrast, other cell types in the superficial, gland acinar, and alveolar epithelia expressed little WT CFTR protein. No ⌬F508 CFTR mature protein or function could be detected in airway specimens freshly excised from a large number of ⌬F508 homozygous subjects, despite an intact ERM complex. In sum, our data demonstrate that WT CFTR is predominantly expressed in ciliated cells, and ⌬F508 CFTR pathogenesis in native tissues, like heterologous cells, reflects loss of normal protein processing.

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Section: Discussionmentioning

confidence: 95%

Section: Discussionmentioning

confidence: 99%

Section: Expression Of ⌬F508 Cftr In Cf Airway Epitheliamentioning

confidence: 99%

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Characterization of Wild-Type and ΔF508 Cystic Fibrosis Transmembrane Regulator in Human Respiratory Epithelia

Kreda

Mall

Mengos

et al. 2005

MBoC

233

210

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“…In contrast to wt and F508del/F508del cells, in which the CFTR protein could be detected at the apical membrane (Figure 3a), apical CFTR staining was significantly reduced in nasal epithelial cells derived from F508del/3905insT compoundheterozygous patients (Figure 3c; Table 1 Effect of CFTR 3905insT at mRNA and protein level J Sanz et al number of cells from F508del homozygous patients have apically localized CFTR (Figure 3b). 21,36,37 Recent studies indicated that the CFTR C-terminus is not required for the biosynthesis and plasma membrane targeting of CFTR, but indispensable for maintaining the stability of the protein. 38 Benharouga et al 39 could also show that an ERAD-similar mechanism involving the proteasome-ubiquitin pathway may be responsible for the faster turnover and the short residence time at the apical membrane of truncated CFTR.…”

Section: Discussionmentioning

confidence: 99%

The CFTR frameshift mutation 3905insT and its effect at transcript and protein level

et al. 2009

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Cystic fibrosis (CF) is one of the most common genetic diseases in the Caucasian population and is characterized by chronic obstructive pulmonary disease, exocrine pancreatic insufficiency, and elevation of sodium and chloride concentrations in the sweat and infertility in men. The disease is caused by mutations in the CF transmembrane conductance regulator (CFTR) gene, which encodes a protein that functions as chloride channel at the apical membrane of different epithelia. Owing to the high genotypic and phenotypic disease heterogeneity, effects and consequences of the majority of the CFTR mutations have not yet been studied. Recently, the frameshift mutation 3905insT was identified as the second most frequent mutation in the Swiss population and found to be associated with a severe phenotype. The frameshift mutation produces a premature termination codon (PTC) in exon 20, and transcripts bearing this PTC are potential targets for degradation through nonsense-mediated mRNA decay (NMD) and/or for exon skipping through nonsense-associated alternative splicing (NAS). Using RT-PCR analysis in lymphocytes and different tissue types from patients carrying the mutation, we showed that the PTC introduced by the mutation does neither elicit a degradation of the mRNA through NMD nor an alternative splicing through NAS. Moreover, immunocytochemical analysis in nasal epithelial cells revealed a significantly reduced amount of CFTR at the apical membrane providing a possible molecular explanation for the more severe phenotype observed in F508del/3905insT compound heterozygotes compared with F508del homozygotes. However, further experiments are needed to elucidate the fate of the 3905insT CFTR in the cell after its biosynthesis.

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“…The most common mutation in CF is the deletion of a phenylalanine residue at position 508 (F508) that causes improper folding of the CFTR protein, resulting in its retention in the endoplasmic reticulum and proteosomal degradation of the majority of the newly synthesized CFTR proteins (Cheng et al, 1990;Kartner et al, 1992;Penque et al, 2000). However, part of the F508-CFTR protein can still mature and reach the cell membrane where it retains some chloride channel function (Bronsveld et al, 2000;Penque et al, 2000;Kopito, 1999).any efforts on CF research are devoted to attempt to rescueF508-CFTR defective trafficking to restore normal epithelial function.…”

Section: Rescue Of F508-cftr Maturation and Membrane Stabilitymentioning

confidence: 99%

VIP as a Corrector of CFTR Trafficking and Membrane Stability

Chappe¹,

Said²

2012

Cystic Fibrosis - Renewed Hopes Through Research

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Cystic Fibrosis F508del Patients Have Apically Localized CFTR in a Reduced Number of Airway Cells

Cited by 89 publications

References 67 publications

Characterization of Wild-Type and ΔF508 Cystic Fibrosis Transmembrane Regulator in Human Respiratory Epithelia

Characterization of Wild-Type and ΔF508 Cystic Fibrosis Transmembrane Regulator in Human Respiratory Epithelia

The CFTR frameshift mutation 3905insT and its effect at transcript and protein level

VIP as a Corrector of CFTR Trafficking and Membrane Stability

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