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fce  (New England Biolabs)


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    Structured Review

    New England Biolabs fce
    Direct measurement of 5′ Cap and poly(A) tail incorporation with Tth-MazF1. ( A ) A schematic of the 5′ Cap and poly(A) tail characterization in <t>Tth-MazF1</t> <t>mRNA</t> digests. ( B ) Heat map depicting the fraction of Cap incorporation in the initial Tth-MazF1 18-nt nucleotide cleavage product of a FLuc mRNA treated with <t>FCE</t> or untreated (NE). Relative quantification of individual species was performed by comparison of the intensity of corresponding monoisotopic masses. ( C ) (Top) A schematic of the predicted Tth-MazF1 cleavage product from the 3′ end of a GFP mRNA with a 60 nt encoded poly(A) tail. (Bottom) Spectra of observed monoisotopic masses between 15 and 28 kDa and corresponding intensities following cleavage of a GFP mRNA with a 60 nt encoded poly(A) tail. Numbers above each peak indicate the annotated length of each oligonucleotide derived from the poly(A) tail. ( D ) Intensity-weighted density plot of the inferred length of poly(A) tails, which were detected in Tth-MazF1 digests of a GFP mRNA with a 60 nt encoded poly(A) tail.
    Fce, supplied by New England Biolabs, used in various techniques. Bioz Stars score: 96/100, based on 146 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
    https://www.bioz.com/result/fce/product/New England Biolabs
    Average 96 stars, based on 146 article reviews
    fce - by Bioz Stars, 2026-05
    96/100 stars

    Images

    1) Product Images from "Systematic screening of archaeal MazF homologs reveals Tth-MazF1, a versatile, sequence-specific ribonuclease from Thermococcus thioreducens"

    Article Title: Systematic screening of archaeal MazF homologs reveals Tth-MazF1, a versatile, sequence-specific ribonuclease from Thermococcus thioreducens

    Journal: Nucleic Acids Research

    doi: 10.1093/nar/gkag338

    Direct measurement of 5′ Cap and poly(A) tail incorporation with Tth-MazF1. ( A ) A schematic of the 5′ Cap and poly(A) tail characterization in Tth-MazF1 mRNA digests. ( B ) Heat map depicting the fraction of Cap incorporation in the initial Tth-MazF1 18-nt nucleotide cleavage product of a FLuc mRNA treated with FCE or untreated (NE). Relative quantification of individual species was performed by comparison of the intensity of corresponding monoisotopic masses. ( C ) (Top) A schematic of the predicted Tth-MazF1 cleavage product from the 3′ end of a GFP mRNA with a 60 nt encoded poly(A) tail. (Bottom) Spectra of observed monoisotopic masses between 15 and 28 kDa and corresponding intensities following cleavage of a GFP mRNA with a 60 nt encoded poly(A) tail. Numbers above each peak indicate the annotated length of each oligonucleotide derived from the poly(A) tail. ( D ) Intensity-weighted density plot of the inferred length of poly(A) tails, which were detected in Tth-MazF1 digests of a GFP mRNA with a 60 nt encoded poly(A) tail.
    Figure Legend Snippet: Direct measurement of 5′ Cap and poly(A) tail incorporation with Tth-MazF1. ( A ) A schematic of the 5′ Cap and poly(A) tail characterization in Tth-MazF1 mRNA digests. ( B ) Heat map depicting the fraction of Cap incorporation in the initial Tth-MazF1 18-nt nucleotide cleavage product of a FLuc mRNA treated with FCE or untreated (NE). Relative quantification of individual species was performed by comparison of the intensity of corresponding monoisotopic masses. ( C ) (Top) A schematic of the predicted Tth-MazF1 cleavage product from the 3′ end of a GFP mRNA with a 60 nt encoded poly(A) tail. (Bottom) Spectra of observed monoisotopic masses between 15 and 28 kDa and corresponding intensities following cleavage of a GFP mRNA with a 60 nt encoded poly(A) tail. Numbers above each peak indicate the annotated length of each oligonucleotide derived from the poly(A) tail. ( D ) Intensity-weighted density plot of the inferred length of poly(A) tails, which were detected in Tth-MazF1 digests of a GFP mRNA with a 60 nt encoded poly(A) tail.

    Techniques Used: Quantitative Proteomics, Comparison, Derivative Assay



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    Direct measurement of 5′ Cap and poly(A) tail incorporation with Tth-MazF1. ( A ) A schematic of the 5′ Cap and poly(A) tail characterization in <t>Tth-MazF1</t> <t>mRNA</t> digests. ( B ) Heat map depicting the fraction of Cap incorporation in the initial Tth-MazF1 18-nt nucleotide cleavage product of a FLuc mRNA treated with <t>FCE</t> or untreated (NE). Relative quantification of individual species was performed by comparison of the intensity of corresponding monoisotopic masses. ( C ) (Top) A schematic of the predicted Tth-MazF1 cleavage product from the 3′ end of a GFP mRNA with a 60 nt encoded poly(A) tail. (Bottom) Spectra of observed monoisotopic masses between 15 and 28 kDa and corresponding intensities following cleavage of a GFP mRNA with a 60 nt encoded poly(A) tail. Numbers above each peak indicate the annotated length of each oligonucleotide derived from the poly(A) tail. ( D ) Intensity-weighted density plot of the inferred length of poly(A) tails, which were detected in Tth-MazF1 digests of a GFP mRNA with a 60 nt encoded poly(A) tail.
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    Image Search Results


    Direct measurement of 5′ Cap and poly(A) tail incorporation with Tth-MazF1. ( A ) A schematic of the 5′ Cap and poly(A) tail characterization in Tth-MazF1 mRNA digests. ( B ) Heat map depicting the fraction of Cap incorporation in the initial Tth-MazF1 18-nt nucleotide cleavage product of a FLuc mRNA treated with FCE or untreated (NE). Relative quantification of individual species was performed by comparison of the intensity of corresponding monoisotopic masses. ( C ) (Top) A schematic of the predicted Tth-MazF1 cleavage product from the 3′ end of a GFP mRNA with a 60 nt encoded poly(A) tail. (Bottom) Spectra of observed monoisotopic masses between 15 and 28 kDa and corresponding intensities following cleavage of a GFP mRNA with a 60 nt encoded poly(A) tail. Numbers above each peak indicate the annotated length of each oligonucleotide derived from the poly(A) tail. ( D ) Intensity-weighted density plot of the inferred length of poly(A) tails, which were detected in Tth-MazF1 digests of a GFP mRNA with a 60 nt encoded poly(A) tail.

    Journal: Nucleic Acids Research

    Article Title: Systematic screening of archaeal MazF homologs reveals Tth-MazF1, a versatile, sequence-specific ribonuclease from Thermococcus thioreducens

    doi: 10.1093/nar/gkag338

    Figure Lengend Snippet: Direct measurement of 5′ Cap and poly(A) tail incorporation with Tth-MazF1. ( A ) A schematic of the 5′ Cap and poly(A) tail characterization in Tth-MazF1 mRNA digests. ( B ) Heat map depicting the fraction of Cap incorporation in the initial Tth-MazF1 18-nt nucleotide cleavage product of a FLuc mRNA treated with FCE or untreated (NE). Relative quantification of individual species was performed by comparison of the intensity of corresponding monoisotopic masses. ( C ) (Top) A schematic of the predicted Tth-MazF1 cleavage product from the 3′ end of a GFP mRNA with a 60 nt encoded poly(A) tail. (Bottom) Spectra of observed monoisotopic masses between 15 and 28 kDa and corresponding intensities following cleavage of a GFP mRNA with a 60 nt encoded poly(A) tail. Numbers above each peak indicate the annotated length of each oligonucleotide derived from the poly(A) tail. ( D ) Intensity-weighted density plot of the inferred length of poly(A) tails, which were detected in Tth-MazF1 digests of a GFP mRNA with a 60 nt encoded poly(A) tail.

    Article Snippet: Briefly, 50 μg of FLuc mRNA was diluted to a final volume of 50 μl in FCE capping buffer (50 mM Tris–HCl, 5 mM KCl, 1 mM MgCl 2 , 1 mM DTT, pH 8.0) containing 200 μM S-adenosylmethionine (SAM), 500 μM GTP, 50 units of FCE, and 200 units of mRNA Cap 2′-O-methyltransferase (NEB, M0366).

    Techniques: Quantitative Proteomics, Comparison, Derivative Assay