Nuclear Factor I in neurons, glia and during the formation of Müller glia-derived progenitor cells in avian, porcine and primate retinas

El‐Hodiri, Heithem M.; Campbell, Warren A.; Kelly, Lisa E.; Hawthorn, Evan C.; Schwartz, M.; Jalligampala, Archana; McCall, Maureen A.; Meyer, Kathrin; Fischer, Andy J.

doi:10.1101/2021.07.13.451621

Cited by 1 publication

(1 citation statement)

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“…Retinal microglia are known to influence the ability of MG to become proliferating MGPCs [56, 67]. Accordingly, we probed scRNA-seq of normal and damaged chick retinas with the microglia intact or ablated by clodronate-liposomes, as originally described in detail in a recent study [68]. More than 95% of the microglia are ablated with 3 days of treatment with clodronate-liposome [39, 56].…”

Section: Resultsmentioning

confidence: 99%

Protein phosphatases regulate the formation of Müller glia-derived progenitor cells in the chick retina

Kelly,

El-Hodiri,

Crider

et al. 2023

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Different kinase-dependent cell signaling pathways are known to play important roles in glia-mediated neuroprotection and reprogramming of Müller glia (MG) into Müller glia-derived progenitor cells (MGPCs) in the retina. However, very little is known about the phosphatases that regulate kinase-dependent signaling in MG. Using single-cell RNA-sequencing (scRNA-seq) databases, we investigated patterns of expression of Dual Specificity Phosphatases (DUSP1/6) and other protein phosphatases in normal and damaged chick retinas. We found thatDUSP1, DUSP6, PPP3CB, PPP3R1andPPPM1A/B/D/E/Gare dynamically expressed by MG and MGPCs in retinas during the process of reprogramming. We find that inhibition of DUSP1/6 and PP2C phosphatases enhances the formation of proliferating MGPCs in damaged retinas and in retinas treated with insulin in FGF2 in the absence of damage. By contrast, inhibition of PP2B phosphatases suppressed the formation of proliferating MGPCs, but increased numbers of proliferating MGPCs in undamaged retinas treated with insulin and FGF2. In damaged retinas, inhibition of DUSP1/6 increased levels of pERK1/2 and cFos in MG whereas inhibition of PP2B’s decreased levels of pStat3 and pS6 in MG. Analyses of scRNA-seq libraries identified numerous differentially activated gene modules in MG in damaged retinas versus MG in retinas treated with insulin+FGF2 suggesting significant differences in kinase-dependent signaling pathways that converge on the formation of MGPCs. Inhibition of phosphatases had no significant effects upon numbers of dying cells in damaged retinas. We conclude that the activity of different protein phosphatases “fine-tune” the cell signaling responses of MG in damaged retinas and during the reprogramming of MG into MGPCs.

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