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Published April 10, 2018 | Published + Supplemental Material
Journal Article Open

Split cGAL, an intersectional strategy using a split intein for refined spatiotemporal transgene control in Caenorhabditis elegans

Abstract

Bipartite expression systems, such as the GAL4-UAS system, allow fine manipulation of gene expression and are powerful tools for interrogating gene function. Recently, we established cGAL, a GAL4-based bipartite expression system for transgene control in Caenorhabditis elegans, where a single promoter dictates the expression pattern of a cGAL driver, which then binds target upstream activation sequences to drive expression of a downstream effector gene. Here, we report a split strategy for cGAL using the split intein gp41-1 for intersectional control of transgene expression. Split inteins are protein domains that associate, self-excise, and covalently ligate their flanking peptides together. We split the DNA binding domain and transcriptional activation domain of cGAL and fused them to the N terminal of gp41-1-N-intein and the C terminal of gp41-1-C-intein, respectively. In cells where both halves of cGAL are expressed, a functional cGAL driver is reconstituted via intein-mediated protein splicing. This reconstitution allows expression of the driver to be dictated by two promoters for refined spatial control or spatiotemporal control of transgene expression. We apply the split cGAL system to genetically access the single pair of MC neurons (previously inaccessible with a single promoter), and reveal an important role of protein kinase A in rhythmic pharyngeal pumping in C. elegans. Thus, the split cGAL system gives researchers a greater degree of spatiotemporal control over transgene expression, and will be a valuable genetic tool in C. elegans for dissecting gene function with finer cell-specific resolution.

Additional Information

© 2018 National Academy of Sciences. Published under the PNAS license. Contributed by Paul W. Sternberg, March 1, 2018 (sent for review November 20, 2017; reviewed by Thomas R. Clandinin and Yishi Jin) We thank D. Tirrell and H. Schwartz for insightful discussion; S. J. Walton and S. Gharib for technical help; members of the P.W.S. laboratory and H. Chiu for editorial comments on the manuscript; and V. Gradinaru and D. Sieburth for sharing reagents. This work was supported by National Institute of Mental Health Grant R21MH115454 (to P.W.S.); National Institute of General Medical Sciences Grant K99GM126137 (to H.W.); a Della Martin Fellowship in Mental Illness (to H.W.); and the Howard Hughes Medical Institute, with which P.W.S. was an investigator. J.L. and A.J.H. were supported by National Institute of General Medical Sciences training Grant T32GM007616, and K.P.Y. was supported by U.S. Army Research Office, Institute for Collaborative Biotechnologies Grant W911NF-09-0001. H.W. and J.L. contributed equally to this work. Author contributions: H.W., J.L., K.P.Y., and P.W.S. designed research; H.W. and J.L. performed research; K.P.Y. and A.J.H. contributed new reagents/analytic tools; H.W. and J.L. analyzed data; and H.W., J.L., and P.W.S. wrote the paper. Data deposition: Some of the plasmids used in this study have been deposited in Addgene (catalog nos. 107130–107137, and 107139, available at https://www.addgene.org/ Paul_Sternberg/). This article contains supporting information online at www.pnas.org/lookup/suppl/doi:10.1073/pnas.1720063115/-/DCSupplemental. The authors declare no conflict of interest.

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Published - 3900.full.pdf

Supplemental Material - pnas.1720063115.sapp.pdf

Supplemental Material - pnas.201720063SI.pdf

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Created:
August 21, 2023
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October 18, 2023