Author response:
The following is the authors’ response to the original reviews.
Reviewer #1 (Recommendations For The Authors):
(1) The description of the wing phenotype that results from combinations of wingless and delex alleles at the bottom of page 4 (figure 1) is quite confusing. Are the trans-hets suppressed to wt or enhanced? The images in the Fig look enhanced.
We thank the reviewer for this thoughtful observation regarding the wing phenotype description in combination with wg and dx alleles. We understand the confusion and appreciate the opportunity to clarify.
In response to the concern raised, the trans-heterozygous indeed enhanced rather than suppressed to wild type. We acknowledge that the description would have been clearer. We have revised the relevant section to explicitly state that trans-heterozygous exhibit an enhanced wing phenotype in the updated version of the manuscript.
(2) Use of Cut as a Wg readout in Fig1 is problematic since it is also a Notch target. Perhaps a more direct measure of Arm activity would be a better choice here, e.g., naked-lacZ.
We appreciate the reviewer’s insightful comment regarding the use of Cut as a Wg readout. The point about being Cut as a Notch target raises a valid concern. To address this issue and provide a more direct measurement of Arm activity, we agree that incorporating a specific Arm readout, such as naked lacZ, would be a more suitable choice.
We will incorporate this valuable feedback into our future research endeavors to augment the comprehensiveness of our study.
(3) The dx allele effects on Sens and Vg in Fig 2C appear greater at two points along the DV margin (arrows). Do these match the expression pattern of dx mRNA?
We thank the reviewer for this thoughtful observation. We understand that the effect of the dx LOF allele on Sens and Vg seems more pronounced at two specific points along the D/V margin. As far as our understanding Dx shows a homogeneous expression pattern throughout the Wg disc which has been reported earlier (Busseau et al., 1994., Mukherjee et al., 2005).
(4) It really looks to my eye that dx loss lowers Wg expression in source cells in Fig 2. To confirm the model that Dx controls the spread of Wg protein, it would be ideal to rule out txnal effects with a wg-lacZ reporter.
We appreciate the reviewer for raising this important point. In the revised version of the manuscript, we have introduced Wg-lacZ staining for both Wg-lacZ/+ and dx152/Y; Wg-lacZ/+ combination in Figure 2. This additional information eliminates the possibility of Deltex influencing Wg transcriptional regulation in source cells, thus reinforcing our hypothesis that the reduction of Deltex leads to a decline in Wg protein levels in the source cells, given Dx essential role in wingless gradient formation.
(5) The drop in DV Wg and expansion of Vg domain in dx mutants seem paradoxical but could be explained by accelerated Wg spread and uptake. This could be tested by depleting the dally-like glypican that promotes long-range Wg diffusion in dx mutants, and seeing if this restores Wg levels at the DV margin.
This is indeed a very thoughtful comment and we thank the reviewer for this insightful suggestion for further exploration. We believe that depleting dally-like glypican in dx mutants could possibly restore Wg levels at the DV margin.
We recognize the importance of this experiment in providing a more comprehensive understanding of the underlying mechanisms, and we will give major emphasis on incorporating this suggestion in our future research.
(6) The authors describe the effect of Dx over-expression as "reducing" the Wg gradient when they actually mean "flattening". Please be careful with this word choice as they mean different things.
We thank the reviewer for the insightful feedback. The suggested modifications have been incorporated into the revised version of the manuscript.
(7) The combined effects of Rab5dn and Dx o/e on Wg protein loc/levels are interesting but need to be followed up by testing whether the endogenous Dx/Rab5 show genetic interactions in control of Wg protein levels/localization.
We acknowledge the reviewer's comment and in addressing it, we wish to highlight that the over-expression of Dx with endogenous Rab5 or Rab7 does not affect Wg protein levels or localization. We have mentioned the supporting data for this control in Figure 5(G, H).
(8) The ability of MG132 to restore Arm levels in en-Dx discs is very promising. However, MG132 will also block Arm degradation by the Slmb-APC destruction complex, so this result could be non-specific. Tests of whether Dx drives poly-ub of Arm, and how much Dx is redundant to Slmb in this role, would be needed to solidify the authors' conclusion.
We thank the reviewer for this insightful comment. We understand that the concern about MG132 blocking Arm degradation by Slmb-APC destruction complex adds an important layer of complexity to the interpretation of the results. We agree with the reviewer's comment that conducting these experiments will indeed offer valuable insight into the specificity of MG132 effects and further strengthen our conclusion.
We are interested to see how future experiments addressing the points raised by the reviewer will shape our understanding of the intricate mechanisms involved in Wg signaling and Arm/-catenin degradation. Once again, we thank the reviewer for the thoughtful engagement with the research, and the comments will undoubtedly stimulate further investigation and discussion in this area.
Reviewer #2 (Recommendations For The Authors):
The work really needs more experiments to further provide a mechanistic understanding and distinguish between direct and indirect action (via Notch signaling) on Wingless, but instead switches in the second half to a second interaction with β-catenin, leaving the conclusions of the first part hanging. More mechanistic information on the cell biology of how Deltex might affect wingless endocytic trafficking directly would be beneficial, for example involving some cell culture experiments where the action of deltex on Notch and wingless could be more clearly separated and a more detailed study of the consequences on wingless trafficking could be explored.
Wingless is secreted into an extracellular compartment and so won't be accessible for a direct interaction with cytoplasmic deltex. Therefore are the authors proposing Deltex interacts with a membrane-bound wingless receptor such as frizzled in order to mediate its effects? These avenues could be explored further experimentally to derive a more mechanistic conclusion.
The colocalisation images are not high resolution and colocalisation is not quantified, and no differences ( +/- Deltex) in wingless subcellular localisation, which would aid mechanistic interpretation, are shown.
We thank the reviewer for the insightful feedback on our work. We appreciate the suggestion for more experiments to provide a mechanistic understanding and to distinguish between direct and indirect actions of Notch on Wingless signaling. We acknowledge the importance of clarifying these aspects and agree that further experiments could help separate the effects of Deltex on Notch and Wingless signaling, allowing for a more detailed examination of their respective trafficking and ubiquitination mechanisms.
We will consider your valuable input in our future research efforts to enhance the comprehensiveness of our study.
Other specific points
Figure 2: Narrowing and broadening of different marker gene expression patterns in dx mutants needs to be quantified so that variation is taken into account and the numbers of wings imaged should be clearly stated.
We greatly appreciate this valuable suggestion from the reviewer. As a response, we have incorporated quantification data to address the observed variations. We have also provided information regarding the number of wing discs that were imaged for the purpose of quantification.
Figure 3: The number of discs imaged in total should be mentioned
We express our appreciation to the reviewer for the input. We have taken their comment into account and have subsequently included details regarding the number of discs imaged in the figure legend section of the manuscript.
Figure 6: There is no description of (E5-E6) in the figure legend. F1 to F5 eye size phenotypes require quantification.
We are grateful to the reviewers for bringing this to our attention. In response, we have included a description of E5-E6 in the figure legend. Also, as per the reviewer’s suggestions, we have incorporated the quantification data of the eye size phenotype.
Discussion
Links between Notch and wingless pathway should be more comprehensively discussed, including previous work that has previously linked Notch/Deltex to β-catenin degradation e.g.
Acar et al. .Sci Rep 2021 Apr 27;11(1):9096. doi: 10.1038/s41598-021-88618-5
Hayward et al. Development 2005 Apr;132(8):1819-30. doi: 10.1242/dev.01724;
Kwon et al Nat Cell Biol 2011 Aug 14;13(10):1244-51. doi: 10.1038/ncb2313.
Sanders et al. PLoS Biol 2009 Aug;7(8):e1000169. doi:10.1371/journal.pbio.1000169. Epub 2009 Aug 11.
The links between endocytic trafficking and wingless gradient formation could also be further discussed eg.
Marois et al. Development 2006 Jan;133(2):307-17.doi: 10.1242/dev.02197. Epub 2005 Dec 14
Yamazaki et al Nat Cell Biol 2016 Apr;18(4):451-7. doi: 10.1038/ncb3325. Epub 2016 Mar 14.
We appreciate the reviewer's valuable suggestions and we have now included these references in the discussion section of the revised manuscript.