Selective loss of RPGRIP1-dependent ciliary targeting of NPHP4, RPGR and SDCCAG8 underlies the degeneration of photoreceptor neurons.

dc.contributor.author

Patil, H

dc.contributor.author

Tserentsoodol, N

dc.contributor.author

Saha, A

dc.contributor.author

Hao, Y

dc.contributor.author

Webb, M

dc.contributor.author

Ferreira, PA

dc.coverage.spatial

England

dc.date.accessioned

2017-10-01T01:57:14Z

dc.date.available

2017-10-01T01:57:14Z

dc.date.issued

2012-07-19

dc.description.abstract

The retinitis pigmentosa GTPase regulator (RPGR) and nephrocystin-4 (NPHP4) comprise two key partners of the assembly complex of the RPGR-interacting protein 1 (RPGRIP1). Mutations in RPGR and NPHP4 are linked to severe multisystemic diseases with strong retinal involvement of photoreceptor neurons, whereas those in RPGRIP1 cause the fulminant photoreceptor dystrophy, Leber congenital amaurosis (LCA). Further, mutations in Rpgrip1 and Nphp4 suppress the elaboration of the outer segment compartment of photoreceptor neurons by elusive mechanisms, the understanding of which has critical implications in uncovering the pathogenesis of syndromic retinal dystrophies. Here we show RPGRIP1 localizes to the photoreceptor connecting cilium (CC) distally to the centriole/basal body marker, centrin-2 and the ciliary marker, acetylated-α-tubulin. NPHP4 abuts proximally RPGRIP1, RPGR and the serologically defined colon cancer antigen-8 (SDCCAG8), a protein thought to partake in the RPGRIP1 interactome and implicated also in retinal-renal ciliopathies. Ultrastructurally, RPGRIP1 localizes exclusively throughout the photoreceptor CC and Rpgrip1(nmf247) photoreceptors present shorter cilia with a ruffled membrane. Strikingly, Rpgrip1(nmf247) mice without RPGRIP1 expression lack NPHP4 and RPGR in photoreceptor cilia, whereas the SDCCAG8 and acetylated-α-tubulin ciliary localizations are strongly decreased, even though the NPHP4 and SDCCAG8 expression levels are unaffected and those of acetylated-α-tubulin and γ-tubulin are upregulated. Further, RPGRIP1 loss in photoreceptors shifts the subcellular partitioning of SDCCAG8 and NPHP4 to the membrane fraction associated to the endoplasmic reticulum. Conversely, the ciliary localization of these proteins is unaffected in glomeruli or tubular kidney cells of Rpgrip1(nmf247), but NPHP4 is downregulated developmentally and selectively in kidney cortex. Hence, RPGRIP1 presents cell type-dependent pathological effects crucial to the ciliary targeting and subcellular partitioning of NPHP4, RPGR and SDCCAG8, and acetylation of ciliary α-tubulin or its ciliary targeting, selectively in photoreceptors, but not kidney cells, and these pathological effects underlie photoreceptor degeneration and LCA.

dc.identifier

https://www.ncbi.nlm.nih.gov/pubmed/22825473

dc.identifier

cddis201296

dc.identifier.eissn

2041-4889

dc.identifier.uri

https://hdl.handle.net/10161/15579

dc.language

eng

dc.publisher

Springer Science and Business Media LLC

dc.relation.ispartof

Cell Death Dis

dc.relation.isversionof

10.1038/cddis.2012.96

dc.subject

Animals

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Autoantigens

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Calcium-Binding Proteins

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Carrier Proteins

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Eye Proteins

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Kidney Tubules

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Mice

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Mutation

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Neoplasm Proteins

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Photoreceptor Connecting Cilium

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Proteins

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Rhodopsin

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Tubulin

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Up-Regulation

dc.title

Selective loss of RPGRIP1-dependent ciliary targeting of NPHP4, RPGR and SDCCAG8 underlies the degeneration of photoreceptor neurons.

dc.type

Journal article

duke.contributor.orcid

Ferreira, PA|0000-0003-4585-1717

pubs.author-url

https://www.ncbi.nlm.nih.gov/pubmed/22825473

pubs.begin-page

e355

pubs.organisational-group

Clinical Science Departments

pubs.organisational-group

Duke

pubs.organisational-group

Ophthalmology

pubs.organisational-group

Pathology

pubs.organisational-group

School of Medicine

pubs.publication-status

Published online

pubs.volume

3

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