Surfactant protein C mutation links postnatal type 2 cell dysfunction to adult disease
Sneha Sitaraman, … , Yan Xu, Timothy E. Weaver
Sneha Sitaraman, … , Yan Xu, Timothy E. Weaver
Published June 17, 2021
Citation Information: JCI Insight. 2021;6(14):e142501. https://doi.org/10.1172/jci.insight.142501.
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Research Article Cell biology Pulmonology

Surfactant protein C mutation links postnatal type 2 cell dysfunction to adult disease

Abstract

Mutations in the gene SFTPC, encoding surfactant protein C (SP-C), are associated with interstitial lung disease in children and adults. To assess the natural history of disease, we knocked in a familial, disease-associated SFTPC mutation, L188Q (L184Q [LQ] in mice), into the mouse Sftpc locus. Translation of the mutant proprotein, proSP-CLQ, exceeded that of proSP-CWT in neonatal alveolar type 2 epithelial cells (AT2 cells) and was associated with transient activation of oxidative stress and apoptosis, leading to impaired expansion of AT2 cells during postnatal alveolarization. Differentiation of AT2 to AT1 cells was also inhibited in ex vivo organoid culture of AT2 cells isolated from LQ mice; importantly, treatment with antioxidant promoted alveolar differentiation. Upon completion of alveolarization, SftpcLQ expression was downregulated, leading to resolution of chronic stress responses; however, the failure to restore AT2 cell numbers resulted in a permanent loss of AT2 cells that was linked to decreased regenerative capacity in the adult lung. Collectively, these data support the hypothesis that susceptibility to disease in adult LQ mice is established during postnatal lung development, and they provide a potential explanation for the delayed onset of disease in patients with familial pulmonary fibrosis.

Authors

Sneha Sitaraman, Emily P. Martin, Cheng-Lun Na, Shuyang Zhao, Jenna Green, Hitesh Deshmukh, Anne-Karina T. Perl, James P. Bridges, Yan Xu, Timothy E. Weaver

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Figure 3

Accumulation of proSP-C in P4 LQ/LQ AT2 cells.

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Accumulation of proSP-C in P4 LQ/LQ AT2 cells. (A) Western blot analyses...
(A) Western blot analyses of 20 μg of AT2 cell lysates separated by SDS-PAGE. Gel was stained after transfer with Coomassie-based instant blue to assess protein loading. (B) Normalization of proSP-C levels in A to total protein using Bio-Rad ImageLab software. (C) Relative Sftpc mRNA levels in isolated AT2 cells obtained by quantitative PCR of 20 ng of cDNA. Data were normalized to Ppia expression. Cycle threshold for Ppia was constant in all genotypes and across developmental time points (Supplemental Figure 5D). RQ, relative quantitation. For B and C, **P < 0.01, ***P < 0.001, ****P < 0.0001 by 2-way ANOVA with Sidak’s multiple comparison test. (D) Lung slices (1 mm) from P3 mice were labeled with [35S] methionine/cysteine for 30 minutes, followed by immunoprecipitation of 4.6 × 106 counts with an antibody directed against the mature SP-C peptide (detects both SP-C proprotein and mature peptide). Lung homogenates were separated by SDS-PAGE, followed by phosphor imaging to detect newly synthesized proSP-C. Top and bottom panels were exposed for 2 and 7 days, respectively. Red box in the bottom portion shows absence of the mature peptide in LQ/LQ lung homogenates. Arrowheads in A and D point to SP-C proprotein. Unedited blots are available online with this article.