Structure-guided point mutations on FusionRed produce a brighter red fluorescent protein

Mukherjee, Srijit; Hung, Sheng-Ting; Douglas, Nancy; Manna, Premashis; Thomas, Connor; Ekrem, Annika; Ae, Palmer; Jimenez, Ralph

doi:10.1101/2020.04.20.051763

Cited by 1 publication

(1 citation statement)

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“…In the meantime, there are definite drawbacks which take from the value of FusionRed as a multipurpose fluorescence tag and call for further improvement of this RFP. Thus, an issue of the modest molecular brightness possessed by FusionRed has been extensively addressed in the elegant studies by the Jimenez lab, where both a directed evolution [17] and semirational design [18] were utilized to engineer the brighter variants of FusionRed (specifically, the FusionRed-MQV [19] shows ~4-fold brightness advantage over the parental RFP, though its emission peak has a 20-nm hypsochromic shift). The high-resolution spatial structure of FusionRed revealed that almost a half of its molecules carries an immature chromophore and possesses a protein backbone cleavage in a vicinity of the chromophore-forming amino acid triad [20].…”

Section: Introductionmentioning

confidence: 99%

The two key substitutions in the chromophore environment of mKate2 to produce an enhanced FusionRed-like red fluorescent protein

Ruchkin,

Gavrikov,

Kolesov

et al. 2023

Preprint

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Red fluorescent proteins (RFPs) can be considered as a probe of choice for living tissue microscopy and whole-body imaging. When choosing a specific RFP variant, the priority may be focused on fluorescence brightness, maturation rate, monomericity, excitation/emission wavelengths, low toxicity, which are rarely combined in optimal way in a single protein. If the additional requirements such as prolonged fluorescence lifetime and/or blinking ability are applied, the available probes repertoire could become surprisingly narrow. Since the whole diversity of the conventional single-component RFPs belongs to just a few phylogenetic lines (with DsRed-, eqFP578- and eqFP611-derived being the major ones), it is not unexpected that their advantageous properties are split between close homologs. In such cases, a systematic mutagenetic analysis focused on variant-specific amino acid residues can shed light on the origins of sibling RFPs distinctness and might be beneficial for consolidation of their strengths in new RFP variants. For instance, the protein FusionRed, although being efficient in the fluorescence labeling due its good monomericity and low cytotoxicity, has undergone a considerable lost in fluorescence brightness/lifetime and received an undesirable alteration in posttranslational chemistry upon its designing from the parental mKate2. In this contribution, we describe a fast-maturing monomeric RFP designed semi-rationally based on the mKate2 and FusionRed templates, outperforming both its parents in brightness, having extended fluorescence lifetime, and showing spontaneous blinking pattern promising for nanoscopy use.

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Section: Introductionmentioning

confidence: 99%