Lipoprotein lipase reaches the capillary lumen in chickens despite an apparent absence of GPIHBP1
Cuiwen He, Xuchen Hu, Rachel S. Jung, Mikael Larsson, Yiping Tu, Sandra Duarte-Vogel, Paul Kim, Norma P. Sandoval, Tara R. Price, Christopher M. Allan, Brian Raney, Haibo Jiang, André Bensadoun, Rosemary L. Walzem, Richard I. Kuo, Anne P. Beigneux, Loren G. Fong, Stephen G. Young
Cuiwen He, Xuchen Hu, Rachel S. Jung, Mikael Larsson, Yiping Tu, Sandra Duarte-Vogel, Paul Kim, Norma P. Sandoval, Tara R. Price, Christopher M. Allan, Brian Raney, Haibo Jiang, André Bensadoun, Rosemary L. Walzem, Richard I. Kuo, Anne P. Beigneux, Loren G. Fong, Stephen G. Young
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Research Article Metabolism

Lipoprotein lipase reaches the capillary lumen in chickens despite an apparent absence of GPIHBP1

Abstract

In mammals, GPIHBP1 is absolutely essential for transporting lipoprotein lipase (LPL) to the lumen of capillaries, where it hydrolyzes the triglycerides in triglyceride-rich lipoproteins. In all lower vertebrate species (e.g., birds, amphibians, reptiles, fish), a gene for LPL can be found easily, but a gene for GPIHBP1 has never been found. The obvious question is whether the LPL in lower vertebrates is able to reach the capillary lumen. Using purified antibodies against chicken LPL, we showed that LPL is present on capillary endothelial cells of chicken heart and adipose tissue, colocalizing with von Willebrand factor. When the antibodies against chicken LPL were injected intravenously into chickens, they bound to LPL on the luminal surface of capillaries in heart and adipose tissue. LPL was released rapidly from chicken hearts with an infusion of heparin, consistent with LPL being located inside blood vessels. Remarkably, chicken LPL bound in a specific fashion to mammalian GPIHBP1. However, we could not identify a gene for GPIHBP1 in the chicken genome, nor could we identify a transcript for GPIHBP1 in a large chicken RNA-seq data set. We conclude that LPL reaches the capillary lumen in chickens — as it does in mammals — despite an apparent absence of GPIHBP1.

Authors

Cuiwen He, Xuchen Hu, Rachel S. Jung, Mikael Larsson, Yiping Tu, Sandra Duarte-Vogel, Paul Kim, Norma P. Sandoval, Tara R. Price, Christopher M. Allan, Brian Raney, Haibo Jiang, André Bensadoun, Rosemary L. Walzem, Richard I. Kuo, Anne P. Beigneux, Loren G. Fong, Stephen G. Young

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Figure 4

Chicken lipoprotein lipase (cLPL) is located along the luminal surface of capillaries.

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Chicken lipoprotein lipase (cLPL) is located along the luminal surface o...
A 9-day-old chicken was given an intravenous injection of 0.7 mg of an Alexa Fluor 555–labeled goat IgG against cLPL (red), 0.5 mg of fluorescein-labeled Lens culinaris agglutinin (Lectin, green), and 0.7 mg of Alexa Fluor 647–labeled nonimmune goat IgG (cyan). After 4 minutes, the chicken was perfused with 50 ml of PBS followed by 30 ml of 3% paraformaldehyde (PFA) in PBS. Liver, white adipose tissue (WAT), heart, and cerebellum were harvested, fixed in 3% PFA, and 50-μm sections of WAT and 10-μm sections of heart, liver, and cerebellum were prepared. The lectin bound to endothelial cells of capillaries and larger blood vessels; the goat IgG against cLPL bound to capillaries but not larger blood vessels (arrows). The nonimmune goat IgG did not bind to blood vessels of the heart, WAT, or cerebellum (indicating an effective perfusion) but as expected did bind to macrophages in the liver. DNA was stained with DAPI (blue). Scale bars: 50 μm.