Ptbp1 deletion does not induce glia-to-neuron conversion in adult mouse retina and brain

Hoang, Thanh; Kim, Dong Won; Appel, Haley; Pannullo, Nicole; Leavey, Patrick J.; Ozawa, Manabu; Zheng, Sika; Yu, Minzhong; Peachey, Neal S.; Kim, Ju-Hyun; Blackshaw, Seth

doi:10.1101/2021.10.04.462784

Cited by 21 publications

(22 citation statements)

References 47 publications

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“…This could reflect the action of cis-regulatory elements that bind transcription factors that promote neuronal-specific expression, the activity of the vector-encoded transcription factors on the GFAP minipromoter, or some combination of the two. Similar conclusions have been drawn following re-examination of claims of astrocyte-to-neuron conversion in brain (Chen et al, 2021;Hoang et al, 2021;Wang et al, 2021a), and these findings raise serious concerns about the accuracy of previously reported claims of AAV-mediated Müller glia-to-neuron conversion (Yao et al, 2018;Zhou et al, 2020;Xiao et al, 2021).…”

Section: Discussionsupporting

confidence: 68%

Ectopic insert-dependent neuronal expression of GFAP promoter-driven AAV constructs in adult mouse retina

Appel

Pannullo

et al. 2022

Preprint

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Direct reprogramming of retinal Muller glia is a promising avenue for replacing photoreceptors and retinal ganglion cells lost to retinal dystrophies. However, questions have recently been raised about the accuracy of studies claiming efficient glia-to-neuron reprogramming in retina that were conducted using GFAP mini promoter-driven adeno-associated virus (AAV) vectors. In this study, we have addressed these questions using GFAP mini promoter-driven AAV constructs to simultaneously overexpress the mCherry reporter and candidate transcription factors predicted to induce glia-to-neuron conversion, in combination with prospective genetic labeling of retinal Muller glia using inducible Cre-dependent GFP reporters. We find that, while control GFAP-mCherry constructs express faithfully in Muller glia, 5 out of 7 transcription factor overexpression constructs tested are predominantly expressed in amacrine and retinal ganglion cells. However, genetic cell lineage analysis shows no evidence for glia-to-neuron conversion. These findings demonstrate strong insert-dependent effects on AAV-based GFAP mini promoter specificity that preclude its use in inferring cell lineage relationships when studying glia-to-neuron conversion in retina.

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Section: Discussionsupporting

confidence: 68%

Ectopic insert-dependent neuronal expression of GFAP promoter-driven AAV constructs in adult mouse retina

Appel

Pannullo

et al. 2022

Preprint

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“…Aldh1l1-CreER T2 ;LSL-YFP transgenic mouse lines exhibit high specificity in astrocyte, with relatively low (4.3%) neuron mislabeling 6,11 . Indeed, three independent groups observed no AtN conversion through Ptbp1 knockdown or knockout in vivo using Aldh1l1-CreER T2 labeling systems 4,6,7 . In contrast, in another common astrocyte labeling systems using GFAP promoter, AtN conversion have been able to occur .…”

Section: Discussionmentioning

confidence: 99%

“…Since the Aldh1l1-CreER T2 ;LSL-YFP transgenic mouse lines exhibit high specificity in astrocyte, with relatively low (4.3%) neuron mislabeling, it is more specific than GFAP promoter 6,13 . Indeed, three independent groups using Aldh1l1-CreER T2 labeling systems and observed no AtN conversion through Ptbp1 knockdown or knockout in vivo 4,6,7 . However, application of an endogenous promoter-driven mGFAP-Cre;LSL-YFP mouse strain enabled stringent, astrocyte-specific YFP expression, which also showed no AtN conversion under Ptbp1 knockdown 6 .…”

Section: Discussionmentioning

confidence: 99%

Ptbp1 knockdown in mouse striatum did not induce astrocyte-to-neuron conversion using HA-tagged labeling system

Yang

Yan

et al. 2022

Preprint

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Conversion of astrocytes to neurons (AtN) is a promising potential strategy for the treatment of neurodegenerative diseases. Recent studies have reported that shRNA-, CasRx-, or ASO-mediated Ptbp1 suppression could reprogram resident astrocytes to neurons. However, some groups have disputed the data interpretation of the reported AtN conversion events. These controversies surrounding AtN conversion may due to differences in the astrocyte fate-mapping systems they applied from that in the original study, i.e., recombinant mouse strains with astrocyte specific reporter constructs versus AAV-based labeling systems. Here, we applied two AAV-based tracing systems to label astrocytes with either a GFAP-driven tdTomato reporter (AAV-GFAP::tdTomato) or GFAP-driven HA-tagged Cas13X (AAV-GFAP::Cas13X-NLS-HA-sgPtbp1) and found conflicting observations of AtN conversion in mouse striatum. Our findings indicated that inconsistent AtN outcomes may arise from different fate-mapping systems between AAV and transgenic mice, as well as through use of different reporter proteins. Thus, the complexity of astrocyte labeling systems warrants careful attention when drawing conclusions about whether AtN conversion occurs.

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“…Besides, Ptbp1 deletion did not make astrocytes trigger any neuron-like potentials, suggesting that their electrophysiological functions were not altered. In addition, by detecting the expression of glia-specific markers, researchers found that Ptbp1-deficient Müller glia retained expression of the glial marker SOX9 and did not detect gene expression characteristic of neurons, indicating that loss of Ptbp1 function did not significantly alter gene expression in Müller glia nor cause these cells to lose their identity ( Hoang et al, 2021 ).…”

Section: Astrocyte Reprogramming Through Trans-differentiationmentioning

confidence: 99%

“…Secondly, previous study stated that knocking down Ptbp1 readily converted glial cells into neurons in young mice but was difficult to achieve in older mice ( Qian et al, 2020 ). On the contrary, the study recently posted in bioRxiv website showing that Ptbp1 deletion does not induce trans-differentiation of astrocytes into neurons in adult mouse retina and brain ( Hoang et al, 2021 ). Controversies in this field have not yet been definitively resolved, suggesting that we should use more rigorous genetic tools in the future to validate the report on the glial-to-neuron reprogramming.…”

Section: Conclusion and Perspectivementioning

confidence: 99%

Astrocyte Reprogramming in Stroke: Opportunities and Challenges

Peng

Lü

Yang

et al. 2022

Front. Aging Neurosci.

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Stroke is a major cause of morbidity and mortality worldwide. In the early stages of stroke, irreversible damage to neurons leads to high mortality and disability rates in patients. However, there are still no effective prevention and treatment measures for the resulting massive neuronal death in clinical practice. Astrocyte reprogramming has recently attracted much attention as an avenue for increasing neurons in mice after cerebral ischemia. However, the field of astrocyte reprogramming has recently been mired in controversy due to reports questioning whether newborn neurons are derived from astrocyte transformation. To better understand the process and controversies of astrocyte reprogramming, this review introduces the method of astrocyte reprogramming and its application in stroke. By targeting key transcription factors or microRNAs, astrocytes in the mouse brain could be reprogrammed into functional neurons. Additionally, we summarize some of the current controversies over the lack of cell lineage tracing and single-cell sequencing experiments to provide evidence of gene expression profile changes throughout the process of astrocyte reprogramming. Finally, we present recent advances in cell lineage tracing and single-cell sequencing, suggesting that it is possible to characterize the entire process of astrocyte reprogramming by combining these techniques.

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Ptbp1 deletion does not induce glia-to-neuron conversion in adult mouse retina and brain

Cited by 21 publications

References 47 publications

Ectopic insert-dependent neuronal expression of GFAP promoter-driven AAV constructs in adult mouse retina

Ectopic insert-dependent neuronal expression of GFAP promoter-driven AAV constructs in adult mouse retina

Ptbp1 knockdown in mouse striatum did not induce astrocyte-to-neuron conversion using HA-tagged labeling system

Astrocyte Reprogramming in Stroke: Opportunities and Challenges

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