Lung epithelial-specific ablation of CCTα. (A) PCR analysis on lungs obtained from Dox-treated perinatal mice. The deleted
Pcyt1a allele (
Pcyt1aΔ/Δ) was detected as a 255-bp PCR product, in contrast to the 301-bp product from the
Pcyt1afl/fl allele. (B) Real time qRT-PCR of phospholipid biosynthetic pathway transcripts in lungs from
Pcyt1aΔ/Δ (black bars) and control (open bars) mice at E18.5. The primers and probes used for detection of CCTα, CCTβ2, CCTβ3, and phosphatidyl ethanolamine
N-methyltransferase are listed by Wang et al. (40). The results are given as mean mRNA levels ± the standard error of the mean (SEM) (**,
P < 0.01;
n = 4) normalized to the level of GAPDH, using the Δ
CT method. Relative expression was calculated based on the cycle number at which fluorescence exceeded the threshold of detection (
CT). Specifically, the
CT for GAPDH was subtracted from that of the target gene for each well (Δ
CT). The percentage of change in gene expression, relative to the reference control group, was defined as 2
−ΔΔCT, where ΔΔ
CT equals the group Δ
CT minus the Δ
CT of the control group. The value for the control lung set at 1. (C) Perinatal lung sections from littermate controls and
Pcyt1aΔ/Δ mice were stained with hematoxylin and eosin. Scale bars, 50 μm. (D) Perinatal lung sections of
Pcyt1aΔ/Δ and control littermate mice were stained with a goat polyclonal antibody against an internal region of the
Pcyt1a gene product (CCTα). The photomicrographs are representative of eight mice per group. Scale bars, 50 μm. (E) Western blots of perinatal mouse lungs from
Pcyt1aΔ/Δ mice and control littermates, using a rabbit polyclonal C-terminal anti-CCTα (45). Quantification of the Western blots (
n ≥ 4 per genotype) was performed using ImageQuant software, and the results are given as means ± SEM (
,
P < 0.01) standardized to the GAPDH loading control and normalized to results for the littermate controls.