Interactions between the budding yeast IQGAP homologue Iqg1p and its targets revealed by a split-EGFP bimolecular fluorescence complementation assay

Pathmanathan, S.; Barnard, E.; Timson, D.J

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dc.contributor.author	Pathmanathan, S.
dc.contributor.author	Barnard, E.
dc.contributor.author	Timson, D.J
dc.date.accessioned	2014-07-17T06:15:34Z
dc.date.accessioned	2022-07-11T08:25:16Z
dc.date.available	2014-07-17T06:15:34Z
dc.date.available	2022-07-11T08:25:16Z
dc.date.issued	2008-10-31
dc.identifier.uri	http://repo.lib.jfn.ac.lk/ujrr/handle/123456789/551
dc.description.abstract	. A split-EGFP based bimolecular fluorescence complementation (BiFC) assay has been used to detect interactions between the Saccharomyces cerevisiae cytoskeletal scaffolding protein Iqg1p and three targets: myosin essential light chain (Mlc1p), calmodulin (Cmd1p) and the small GTPase Cdc42p. The format of the BiFC assay used ensures that the proteins are expressed at wild type levels thereby avoiding artefacts due to overexpression. This is the first direct in vivo detection of these interactions; in each case, the complex is localised to discrete regions of the yeast cytoplasm. The labelling with EGFP fragments results in changes in growth kinetics, cell size and budding frequency. This is partly due to the reassembled EGFP locking the complexes into essentially permanent interactions. The consequences of this for Iqg1p interactions and BiFC assays in general are discussed.	en_US
dc.language.iso	en	en_US
dc.publisher	No longer published by Elsevier	en_US
dc.title	Interactions between the budding yeast IQGAP homologue Iqg1p and its targets revealed by a split-EGFP bimolecular fluorescence complementation assay	en_US
dc.type	Article	en_US