Highly stable and efficient mRNA templates for mRNA-protein fusions and C-terminally labeled proteins

Miyamoto‐Sato, Etsuko; Takashima, Hideaki; Fuse, Shinichiro; Sue, Kaori; Ishizaka, Masamichi; Tateyama, Seiji; Horisawa, Kenichi; Sawasaki, Tatsuya; Endo, Yaeta; Yanagawa, Hiroshi

doi:10.1093/nar/gng078

Cited by 54 publications

(82 citation statements)

References 24 publications

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“…20 Briefly, the purified DNA was transcribed with a RiboMax large-scale RNA production system-SP6 (Promega). The resulting RNA was purified with an RNeasy mini kit (Qiagen) and ligated with polyethylene glycol (PEG)-Puro spacer [p(dCp) 2 -T(Fluor)p-PEGp-(dCp) 2 -puromycin] using T4 RNA ligase (Takara).…”

Section: Tgggcgagaccgctcgaggttc-3mentioning

confidence: 99%

“…20,21 In the mRNA display technique, each mRNA in a library is covalently bound to its corresponding protein through puromycin, 22,23 but mRNA sequences containing a stop codon or frameshift cannot form mRNA-protein conjugates or cannot be properly translated to generate the C-terminal tag, respectively. Thus, they can be washed away in affinity selection based on a property of the peptide portion.…”

Section: Introductionmentioning

confidence: 99%

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Comparative characterization of random‐sequence proteins consisting of 5, 12, and 20 kinds of amino acids

Tanaka¹,

Doi²,

Takashima³

et al. 2010

Protein Science

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Screening of functional proteins from a random-sequence library has been used to evolve novel proteins in the field of evolutionary protein engineering. However, random-sequence proteins consisting of the 20 natural amino acids tend to aggregate, and the occurrence rate of functional proteins in a random-sequence library is low. From the viewpoint of the origin of life, it has been proposed that primordial proteins consisted of a limited set of amino acids that could have been abundantly formed early during chemical evolution. We have previously found that members of a random-sequence protein library constructed with five primitive amino acids show high solubility (Doi et al., Protein Eng Des Sel 2005;18:279-284). Although such a library is expected to be appropriate for finding functional proteins, the functionality may be limited, because they have no positively charged amino acid. Here, we constructed three libraries of 120-amino acid, random-sequence proteins using alphabets of 5, 12, and 20 amino acids by preselection using mRNA display (to eliminate sequences containing stop codons and frameshifts) and characterized and compared the structural properties of random-sequence proteins arbitrarily chosen from these libraries. We found that random-sequence proteins constructed with the 12-member alphabet (including five primitive amino acids and positively charged amino acids) have higher solubility than those constructed with the 20-member alphabet, though other biophysical properties are very similar in the two libraries. Thus, a library of moderate complexity constructed from 12 amino acids may be a more appropriate resource for functional screening than one constructed from 20 amino acids.

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Section: Tgggcgagaccgctcgaggttc-3mentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Comparative characterization of random‐sequence proteins consisting of 5, 12, and 20 kinds of amino acids

Tanaka¹,

Doi²,

Takashima³

et al. 2010

Protein Science

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show abstract

“…Conventionally, the proteins have been expressed in Escherichia coli, purified to homogeneity, and then fluorescently labelled by chemical modification methods, but the expression and purification of large numbers of proteins is a daunting task. As an approach to overcome this problem, a simple method for in vitro fluorescencelabelling of proteins using a derivative of puromycin was developed in our laboratory (7)(8)(9)(10)(11)(12), and the method was also applied to the fluorescence labelling of newly synthesized proteins in living cells (13). Since our method relies on incorporation of a fluorescent puromycin analogue into the C-terminus of the full-length protein during protein synthesis on ribosomes, the expression and labelling steps are synchronized and a purification process before labelling is unnecessary.…”

Section: Introductionmentioning

confidence: 99%

“…The yield of fluorescently labelled proteins is enhanced by the use of mRNA without a stop codon (Fig. 1C) (7,10), but many cDNA collections contain stop codons and their elimination usually requires a large set of oligo DNA primers. Agafonov et al (14) reported that the inactivation of release factor 1 (RF1) leads to better incorporation of puromycin using template mRNA with a UAG stop codon (Fig.…”

Section: Introductionmentioning

confidence: 99%

High-throughput Fluorescence Labelling of Full-length cDNA Products Based on a Reconstituted Translation System

Kawahashi

Doi

Oishi

et al. 2006

Journal of Biochemistry

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Although recent advances in fluorescence-based technologies, such as protein microarrays, have made it possible to analyse more than 10,000 proteins at once, there is a bottleneck in the step of preparation of large numbers of fluorescently labelled proteins for the comprehensive analysis of protein-protein interactions. Here we describe two independent methods for high-throughput fluorescence-labelling of full-length cDNA products at their C-termini using a reconstituted translation system containing fluorescent puromycin. For the first method, release factor-free systems were used. For the second method, stop codons were excluded from cDNAs by using a common mismatch primer in mutagenic PCR. These methods yielded large numbers of labelled proteins from cDNA sets of various organisms, such as mouse, yeast and Escherichia coli.

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“…Two approaches recently used to identify protein binding partners are mRNA display techniques, such as mRNA-protein fusions (17)(18)(19)(20)(21) and in vitro virus, based on cell-free co-translation and affinity selection (22)(23)(24) and tandem affinity purification (TAP)-mass spectrometry methods. These methods are well suited for identifying the components of complexes that form in near physiological conditions.…”

mentioning

confidence: 99%

Identification of Novel SHPS-1-associated Proteins and Their Roles in Regulation of Insulin-like Growth Factor-dependent Responses in Vascular Smooth Muscle Cells

Shen

Radhakrishnan

et al. 2009

Molecular & Cellular Proteomics

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Tyrosine phosphatase non-receptor type substrate-1 (SHPS-1), a transmembrane protein, plays a vital role in cell migration and proliferation. Our previous studies have shown that insulin-like growth factor-I (IGF-I) stimulates SHPS-1 phosphorylation, leading to recruitment of SHP-2, c-Src, Shc, and Grb2⅐p85 to phosphorylated SHPS-1. Assembly of this signaling complex is required for optimal stimulation of both mitogen-activated protein and phosphatidylinositol 3-kinase pathways. The main aim of the present study was to identify novel proteins that interacted with the cytoplasmic domain of SHPS-1 (SHPS-1/CD) in response to IGF-I stimulation and define the role of these interactions in mediating specific biological functions. We performed a functional proteomic screening to identify SHPS-1 binding partners using combination of mRNA display and the tandem affinity purification-tag methods. Screening identified a number of proteins not previously known to interact with phosphorylated SHPS-1/CD. These novel SHPS-1 binding partners represent several functional categories including heat shock proteins, protein kinases and phosphatases, and proteins that regulate transcription or translation. In Vivo and in vitro studies suggested that most of the proteins bound to SHPS-1 via binding to one of the four SH2 domain containing proteins, SHP-2, CTK, SUPT6H, and STAT1, that directly bound to SHPS-1. Although the binding of most of these proteins to SHPS-1 was positively regulated by IGF-I, a few were negatively regulated, suggesting differential regulation of protein complexes assembled on SHPS-1/CD in response to IGF-I. Further studies showed that truncation of SHPS-1/CD significantly impaired IGF-I-dependent AKT signal transduction and subsequent biological functions including cell survival, protein synthesis, protein aggregation, and prevention of apoptosis. The results emphasize the importance of formation of SHPS-1 signaling complex induced by IGF-I and provide novel insights into our knowledge of the role of this molecular scaffold in regulation of IGF

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Highly stable and efficient mRNA templates for mRNA-protein fusions and C-terminally labeled proteins

Cited by 54 publications

References 24 publications

Comparative characterization of random‐sequence proteins consisting of 5, 12, and 20 kinds of amino acids

Comparative characterization of random‐sequence proteins consisting of 5, 12, and 20 kinds of amino acids

High-throughput Fluorescence Labelling of Full-length cDNA Products Based on a Reconstituted Translation System

Identification of Novel SHPS-1-associated Proteins and Their Roles in Regulation of Insulin-like Growth Factor-dependent Responses in Vascular Smooth Muscle Cells

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