2017
DOI: 10.1073/pnas.1701088114
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Evolutionary steps involving counterion displacement in a tunicate opsin

Abstract: Ci-opsin1 is a visible light-sensitive opsin present in the larval ocellus of an ascidian, Ciona intestinalis. This invertebrate opsin belongs to the vertebrate visual and nonvisual opsin groups in the opsin phylogenetic tree. Ci-opsin1 contains candidate counterions (glutamic acid residues) at positions 113 and 181; the former is a newly acquired position in the vertebrate visual opsin lineage, whereas the latter is an ancestral position widely conserved among invertebrate opsins. Here, we show that Glu113 an… Show more

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Cited by 29 publications
(36 citation statements)
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“…2 and S5 ) reveal an overall homogenous sample before as well as after light irradiation. The photoproduct composition is slightly more heterogeneous as found in other bistable opsins ( 29 , 30 ), likely resembling one of their features.
Figure 2 HPLC analysis of retinal oximes.
…”
Section: Resultsmentioning
confidence: 66%
“…2 and S5 ) reveal an overall homogenous sample before as well as after light irradiation. The photoproduct composition is slightly more heterogeneous as found in other bistable opsins ( 29 , 30 ), likely resembling one of their features.
Figure 2 HPLC analysis of retinal oximes.
…”
Section: Resultsmentioning
confidence: 66%
“…Our study further identifies an arginine at position 186 as critical for the counterion displacement in JellyOp. Whereas E181 has been shown to interact with the Schiff base in the active state of vertebrate ciliary opsins ( 35 ) and even act as a synergistic counterion with E113 in a recently described tunicate opsin ( 36 ), R186 appears to isolate E181 from the PSB of JellyOp, inhibiting its ability to act as a counterion. It follows that the evolution of cubozoan opsins was characterized by accumulation of both E94 and R186.…”
Section: Discussionmentioning
confidence: 99%
“…Consequently, the plasmid encoded a cDNA with a hexahistidine-tag at the C-terminus. Mutant genes were constructed using the QuickChange site-directed mutagenesis method, the SLiCE method or an In-Fusion Cloning Kit according, to the manufacturer’s instructions as previously described [ 25 , 27 , 28 ]. Proteins were expressed in E. coli BL21 (DE3) cells using the same experimental procedures as previously described [ 25 ].…”
Section: Methodsmentioning
confidence: 99%