mCherry contains a fluorescent protein isoform that interferes with its reporter function

Fages-Lartaud, Maxime; Tietze, Lisa; Elie, Florence; Lale, Rahmi; Hohmann‐Marriott, Martin F.

doi:10.3389/fbioe.2022.892138

Cited by 10 publications

(16 citation statements)

References 44 publications

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“…Coinciding with our observation of the expression of mNG from a rudimental methionine at the end of a GFP-derived N-terminus, it was also described for mCherry in a preprint by Fages-Lartaud and colleagues 30 . These scientists used an E. coli optimised version of mCh, which contained a similar RBS upstream of Met10.…”

Section: Discussionsupporting

confidence: 74%

“…Another concern we wish to address is that it is often (almost) undecipherable from publications whether fluorescent proteins have been codon-optimized and to what extent. The amino acid sequence and, therefore the resulting protein may be the same, but as this study and the work of Fages-Lartaud and colleagues 30 shows: it does matter and should be reported more clearly. sfTq2 ox and sfTq2 oxopt have the same amino acid sequence and can therefore consider to be the same protein: however, their expression in E. coli differs hugely.…”

Section: Discussionsupporting

confidence: 55%

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Optimising expression of the large dynamic range FRET pair mNeonGreen and superfolder mTurquoise2ox for use in the Escherichia coli cytoplasm

Mertens

Blaauwen

2022

Sci Rep

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The fluorescent proteins superfolder mTurquoise2ox (sfTq2ox) and mNeonGreen function excellently in mammalian cells, but are not well expressed in E. coli when forming the N-terminus of constructs. Expression was increased by decreasing structures at the start of their coding sequences in the mRNA. Unfortunately, the expression of mNeonGreen started from methionine at position ten as optimisation introduced an alternative RBS in the GFP N-terminus of mNeonGreen. The original start-codon was not deleted, which caused the expression of isomers starting at the original start-codon and at the start-codon at the beginning of the GFP N-terminus. By omitting the GFP N-terminus of mNeonGreen and optimising the structure of its mRNA, the expression of a mixture of isomers was avoided, and up to ~ 50-fold higher expression rates were achieved for mNeonGreen. Both fluorescent proteins can now be expressed at readily detectable levels in E. coli and can be used for various purposes. One explored application is the detection of in-cell protein interactions by FRET. mNeonGreen and sfTq2ox form a FRET pair with a larger dynamic range than commonly used donor–acceptor pairs, allowing for an excellent signal-to-noise ratio, which supports the detection of conformational changes that affect the distance between the interacting proteins.

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Section: Discussionsupporting

confidence: 74%

Section: Discussionsupporting

confidence: 55%

Optimising expression of the large dynamic range FRET pair mNeonGreen and superfolder mTurquoise2ox for use in the Escherichia coli cytoplasm

Mertens

Blaauwen

2022

Sci Rep

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“…Alternative translative start sites are a common issue occurring with N-terminal protein tags and fluorescent proteins. 66,68 This result support the hypothesis of an alternative start codon close to the gene start producing a GFP isoform. Nevertheless, this artifact does not interfere with the conclusion regarding the in vivo cleavage performance of DnaB-GFP.…”

Section: Design Of the Standard Intein Gene Expression Ramp (Siger)supporting

confidence: 83%

“…For DnaB-mCherry , a first observation is that fluorescence levels are generally higher than expected from the DnaB-GFP range, although the relative strength ranking of GES remained the same (Figure a). This slight mCherry overexpression could be due to the newly identified alternative translation start site of mCherry that produces a short functional protein isoform . The short mCherry isoform produces significant background fluorescence when the reporter is used as a C-terminal fusion partner.…”

Section: Results and Discussionmentioning

confidence: 99%

“…This slight mCherry overexpression could be due to the newly identified alternative translation start site of mCherry that produces a short functional protein isoform. 66 The short mCherry isoform produces significant background fluorescence when the reporter is used as a C-terminal fusion partner. Although the background fluorescence is supposedly the same across strains, the production of the short mCherry isoform blurs the relative differences in the expression range.…”

Section: Resultsmentioning

confidence: 99%

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Standard Intein Gene Expression Ramps (SIGER) for Protein-Independent Expression Control

et al. 2023

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Coordination of multigene expression is one of the key challenges of metabolic engineering for the development of cell factories. Constraints on translation initiation and early ribosome kinetics of mRNA are imposed by features of the 5′UTR in combination with the start of the gene, referred to as the "gene ramp", such as rare codons and mRNA secondary structures. These features strongly influence the translation yield and protein quality by regulating the ribosome distribution on mRNA strands. The utilization of genetic expression sequences, such as promoters and 5′UTRs in combination with different target genes, leads to a wide variety of gene ramp compositions with irregular translation rates, leading to unpredictable levels of protein yield and quality. Here, we present the Standard Intein Gene Expression Ramp (SIGER) system for controlling protein expression. The SIGER system makes use of inteins to decouple the translation initiation features from the gene of a target protein. We generated sequence-specific gene expression sequences for two inteins (DnaB and DnaX) that display defined levels of protein expression. Additionally, we used inteins that possess the ability to release the C-terminal fusion protein in vivo to avoid the impairment of protein functionality by the fused intein. Overall, our results show that SIGER systems are unique tools to mitigate the undesirable effects of gene ramp variation and to control the relative ratios of enzymes involved in molecular pathways. As a proof of concept of the potential of the system, we also used a SIGER system to express two difficult-toproduce proteins, GumM and CBM73.

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A GAPDH serotonylation system couples CD8+ T cell glycolytic metabolism to antitumor immunity

Wang,

Fu,

Yuan

et al. 2024

Molecular Cell

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mCherry contains a fluorescent protein isoform that interferes with its reporter function

Cited by 10 publications

References 44 publications

Optimising expression of the large dynamic range FRET pair mNeonGreen and superfolder mTurquoise2ox for use in the Escherichia coli cytoplasm

Optimising expression of the large dynamic range FRET pair mNeonGreen and superfolder mTurquoise2ox for use in the Escherichia coli cytoplasm

Standard Intein Gene Expression Ramps (SIGER) for Protein-Independent Expression Control

A GAPDH serotonylation system couples CD8+ T cell glycolytic metabolism to antitumor immunity

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