Opto-RhoGEFs: an optimized optogenetic toolbox to reversibly control Rho GTPase activity on a global to subcellular scale, enabling precise control over vascular endothelial barrier strength

Reviewer #1 (Public Review):

This manuscript by Mahlandt, et al. presents a significant advance in the manipulation of endothelial barriers with spatiotemporal precision, and in the use of optogenetics to manipulate cell signaling in vascular biology more generally. The authors establish the role of Rho-family GTPases in controlling the cytoskeletal-plasma membrane interface as it relates to endothelial barrier integrity and function and adequately motivate the need for optogenetic tools for global and local signaling manipulation to study endothelial barriers.

Throughout the work, the optogenetic assays are conceptualized, described, and executed with exceptional attention to detail, particularly as it relates to potential confounding factors in data analysis and interpretation. Comparison across experimental setups in optogenetics is notoriously fraught, and the authors' control experiments and measurements to ensure equal light delivery and pathway activation levels across applications are very thorough. In demonstrating how these new opto-GEFs can be used to alter vascular barrier strength, the authors cleverly use fluorescent-labeled dextran polymers of different sizes and ECIS experiments to demonstrate the physiological relevance of BOEC monolayers to in vivo blood vessels. Of particular note, the resiliency of the system to multiple stimulation cycles and longer time course experiments is promising for use in vascular leakage studies.

Given that dozens of Rho GTPase-activating GEFs exist, an expanded rationale for the selection of p63, ITSN1, and TIAM1 in the form of discussion and literature citations would be helpful to motivate their selection as protein effectors in the engineered tools. Extensive tool engineering studies demonstrate the superiority of iLID over optogenetic eMags or rapamycin-based chemogenetic tools for these purposes. However, as the utility of iLID and eMags has been demonstrated for the manipulation of a variety of signaling pathways, the iSH-Akt demonstration does not seem necessary for these systems.

The demonstration of orthogonality in GTPase- and VE-cadherin-blocking antibody-mediated barrier function decreases and is compelling, even without full elucidation of the role of cell size or overlap in barrier strength. The discussion section presents a mature and thoughtful description of the limitations, remaining questions, and potential opportunities for the tools and technology developed in this work. Importantly, this manuscript demonstrates a commitment to scientific transparency in the ways in which the data are visualized, the methods descriptions, and the reagent and code sharing it presents, allowing others to utilize these tools to their full potential.

Reviewer #2 (Public Review):

This manuscript reports on the use of Optogenetics to influence endothelial barrier integrity by light. Light-induced membrane recruitment of GTPase GEFs is known to stimulate GTPases and modulate cell shape, and here this principle is used to modulate endothelial barrier function. It shows that Rac and CDc42 activating constructs enhance barrier function and do this even when a major junctional adhesion molecule, VE-cadherin, is blocked. Activation of Rac and Cdc42 enhanced lamellipodia formation and cellular overlaps, which could be the basis for the increase in barrier integrity.

The authors aimed at developing a light-driven technique with which endothelial barrier integrity can be modulated on the basis of activating certain GTPases. They succeeded in using optogenetic tools that recruit GEF exchange domains to membranes upon light induction in endothelial cell monolayers. Similar tools were in principle known before to modulate cell shape/morphology upon light induction but were used here for the first time as regulators of endothelial barrier integrity. In this way, it was shown that the activation of Cdc42 and Rac can increase barrier integrity even if VE-cadherin, a major adhesion molecule of endothelial junctions, is blocked. Although it was shown before that stimulation of the S1P1 receptor or of Tie-2 can enhance endothelial barrier integrity in dependence on Cdc42 or Rac1 and can do this independent of VE-cadherin, the current study shows this with tools directly targeting these GTPases.

Furthermore, this study presents very valuable tools. The immediate and repeatable responses of barrier integrity changes upon light-on and light-off switches are fascinating and impressive. It will be interesting to use these tools in the future in the context of analyzing other mechanisms which also affect endothelial barrier function and modulate the formation of endothelial adherens junctions.

Reviewer #3 (Public Review):

Mahlandt et al. report the design and proof of concept of Opto-RhoGEF, a new set of molecular tools to control the activation by light of the three best-known members of the Rho GTPase family, RhoA, Rac1, and Cdc42.

The study is based on the optogenetically-controlled activation of chimeric proteins that target the plasma membrane guanine nucleotide exchange factors (GEFs) domains, which are natural activators specific for each of these three Rho GTPases. Membrane-targeted GEFs encounter and activate endogenous Rho proteins. Further investigation into the effect of these tools on RhoGTPase signaling would have strengthened the report.

These three Opto-RhoGEFs are reversible and enable the precise spatiotemporal control of Rho-regulated processes, such as endothelial barrier function, cell contraction, and plasma membrane extension. Hence, these molecular tools will be of broad interest to cell biologists interested in this family of GTPases.

Mahlandt et al. design and characterize three new optogenetic tools to artificially control the activation of the RhoA, Rac1, and Cdc42 by light. These three Rho GTPases are master regulators of the actin cytoskeleton, thereby regulating cell-cell contact stability or actin-mediated contraction and membrane protrusions.

The main strength of this new experimental resource lies in the fact that, to date, few tools controlling Rho activation by reversibly targeting Rho GEFs to the plasma membrane are available. In addition, a comparative analysis of the three Opto-RhoGEFs adds value and further strengthens the results, given the fact that each Opto-GEF produces different (and somehow expected) effects, which suggest specific GTPase activation. The design of the tools is correct, although the membrane targeting could be improved, since the Lck N-terminus used to construct the recombinant proteins contains myristoylation and palmitoylation sites, which have the potential to target the chimeric protein to lipid rafts. As a consequence, this may not evenly translocate these Rho-activating domains.

An additional technical feature that must be highlighted is an elegant method to activate Opto-RhoGEFs in cultured cells, independent of laser and microscopes, by using led strips, which notably expands the possibilities of this resource, potentially allowing biochemical analyses in large numbers of cells.

The experimental evidence clearly indicates that the authors have achieved their aim and designed very useful tools. However, they should have taken more advantage of this remarkable technical advance and investigated in further detail the spatiotemporal dynamics of Rho-mediated signaling. Although the manuscript is a "tool and resource", readers may have better grasped the potential benefits of tuning GTPase activity with this tool by learning about some original and quantitative insights of RhoA, Rac1, and Cdc42 function.

One of such insights may have come from the set of data regarding the contribution of adherens junctions. The effect of other endothelial cell-cell junctions, such as tight junctions, may also contribute to barrier function, as well as junctional independent, cell-substratum adhesion. These optogenetic tools will undoubtedly impact these future studies and help decipher whether these other adhesion events that are important for endothelial barrier integrity are also under the control of these three GTPases. Overall, the manuscript is sound and presents new and convincing experimental strategies to apply optogenetics to the field of Rho GTPases.