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Why does the zebrafish cloche mutant develop lens cataract?
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Abstract
The zebrafish has become a valuable model for examining ocular lens development, physiology and disease. The zebrafish
cloche
mutant, first described for its loss of hematopoiesis, also shows reduced eye and lens size, interruption in lens cell differentiation and a cataract likely caused by abnormal protein aggregation. To facilitate the use of the
cloche
mutant for studies on cataract development and prevention we characterized variation in the lens phenotype, quantified changes in gene expression by qRT-PCR and RNA-Seq and compared the ability of two promoters to drive expression of introduced proteins into the
cloche
lens. We found that the severity of
cloche
embryo lens cataract varied, while the decrease in lens diameter and retention of nuclei in differentiating lens fiber cells was constant. We found very low expression of both αB-crystallin genes (
cryaba
and
cryabb
) at 4 days post fertilization (dpf) by both qRT-PCR and RNA-Seq in
cloche, cloche
sibling and wildtype embryos and no significant difference in αA-crystallin (
cryaa
) expression. RNA-Seq analysis of 4 dpf embryos identified transcripts from 25,281 genes, with 1,329 showing statistically significantly different expression between
cloche
and wildtype samples. Downregulation of eight lens β- and γM-crystallin genes and 22 retinal related genes may reflect a general reduction in eye development and growth. Six stress response genes were upregulated. We did not find misregulation of any known components of lens development gene regulatory networks. These results suggest that the
cloche
lens cataract is not caused by loss of αA-crystallin or changes to lens gene regulatory networks. Instead, we propose that the cataract results from general physiological stress related to loss of hematopoiesis. Our finding that the zebrafish αA-crystallin promoter drove strong GFP expression in the
cloche
lens demonstrates its use as a tool for examining the effects of introduced proteins on lens crystallin aggregation and cataract prevention.
Title: Why does the zebrafish
cloche
mutant develop lens cataract?
Description:
Abstract
The zebrafish has become a valuable model for examining ocular lens development, physiology and disease.
The zebrafish
cloche
mutant, first described for its loss of hematopoiesis, also shows reduced eye and lens size, interruption in lens cell differentiation and a cataract likely caused by abnormal protein aggregation.
To facilitate the use of the
cloche
mutant for studies on cataract development and prevention we characterized variation in the lens phenotype, quantified changes in gene expression by qRT-PCR and RNA-Seq and compared the ability of two promoters to drive expression of introduced proteins into the
cloche
lens.
We found that the severity of
cloche
embryo lens cataract varied, while the decrease in lens diameter and retention of nuclei in differentiating lens fiber cells was constant.
We found very low expression of both αB-crystallin genes (
cryaba
and
cryabb
) at 4 days post fertilization (dpf) by both qRT-PCR and RNA-Seq in
cloche, cloche
sibling and wildtype embryos and no significant difference in αA-crystallin (
cryaa
) expression.
RNA-Seq analysis of 4 dpf embryos identified transcripts from 25,281 genes, with 1,329 showing statistically significantly different expression between
cloche
and wildtype samples.
Downregulation of eight lens β- and γM-crystallin genes and 22 retinal related genes may reflect a general reduction in eye development and growth.
Six stress response genes were upregulated.
We did not find misregulation of any known components of lens development gene regulatory networks.
These results suggest that the
cloche
lens cataract is not caused by loss of αA-crystallin or changes to lens gene regulatory networks.
Instead, we propose that the cataract results from general physiological stress related to loss of hematopoiesis.
Our finding that the zebrafish αA-crystallin promoter drove strong GFP expression in the
cloche
lens demonstrates its use as a tool for examining the effects of introduced proteins on lens crystallin aggregation and cataract prevention.
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