Literature DB >> 30346377

Interactome-Seq: A Protocol for Domainome Library Construction, Validation and Selection by Phage Display and Next Generation Sequencing.

Maria Felicia Soluri1, Simone Puccio2, Giada Caredda2, Giorgio Grillo3, Vito Flavio Licciulli3, Arianna Consiglio3, Paolo Edomi4, Claudio Santoro1, Daniele Sblattero5, Clelia Peano6.   

Abstract

Folding reporters are proteins with easily identifiable phenotypes, such as antibiotic resistance, whose folding and function is compromised when fused to poorly folding proteins or random open reading frames. We have developed a strategy where, by using TEM-1 β-lactamase (the enzyme conferring ampicillin resistance) on a genomic scale, we can select collections of correctly folded protein domains from the coding portion of the DNA of any intronless genome. The protein fragments obtained by this approach, the so called "domainome", will be well expressed and soluble, making them suitable for structural/functional studies. By cloning and displaying the "domainome" directly in a phage display system, we have showed that it is possible to select specific protein domains with the desired binding properties (e.g., to other proteins or to antibodies), thus providing essential experimental information for gene annotation or antigen identification. The identification of the most enriched clones in a selected polyclonal population can be achieved by using novel next-generation sequencing technologies (NGS). For these reasons, we introduce deep sequencing analysis of the library itself and the selection outputs to provide complete information on diversity, abundance and precise mapping of each of the selected fragment. The protocols presented here show the key steps for library construction, characterization, and validation.

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Year:  2018        PMID: 30346377      PMCID: PMC6235410          DOI: 10.3791/56981

Source DB:  PubMed          Journal:  J Vis Exp        ISSN: 1940-087X            Impact factor:   1.355


  29 in total

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2.  Selecting open reading frames from DNA.

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Review 3.  Two-hybrid technologies in proteomics research.

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Journal:  Biochim Biophys Acta       Date:  2002-01-15

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Authors:  Yuji Nakai; Yoshitaka Nomura; Toshihiro Sato; Akiko Shiratsuchi; Yoshinobu Nakanishi
Journal:  J Biochem       Date:  2005-05       Impact factor: 3.387

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7.  A scaleable and integrated crystallization pipeline applied to mining the Thermotoga maritima proteome.

Authors:  Michael DiDonato; Ashley M Deacon; Heath E Klock; Daniel McMullan; Scott A Lesley
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8.  Selecting soluble/foldable protein domains through single-gene or genomic ORF filtering: structure of the head domain of Burkholderia pseudomallei antigen BPSL2063.

Authors:  Louise J Gourlay; Clelia Peano; Cecilia Deantonio; Lucia Perletti; Alessandro Pietrelli; Riccardo Villa; Elena Matterazzo; Patricia Lassaux; Claudio Santoro; Simone Puccio; Daniele Sblattero; Martino Bolognesi
Journal:  Acta Crystallogr D Biol Crystallogr       Date:  2015-10-31

9.  Filtering "genic" open reading frames from genomic DNA samples for advanced annotation.

Authors:  Sara D'Angelo; Nileena Velappan; Flavio Mignone; Claudio Santoro; Daniele Sblattero; Csaba Kiss; Andrew R M Bradbury
Journal:  BMC Genomics       Date:  2011-06-15       Impact factor: 3.969

10.  edgeR: a Bioconductor package for differential expression analysis of digital gene expression data.

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  1 in total

1.  InteractomeSeq: a web server for the identification and profiling of domains and epitopes from phage display and next generation sequencing data.

Authors:  Simone Puccio; Giorgio Grillo; Arianna Consiglio; Maria Felicia Soluri; Daniele Sblattero; Diego Cotella; Claudio Santoro; Sabino Liuni; Gianluca De Bellis; Enrico Lugli; Clelia Peano; Flavio Licciulli
Journal:  Nucleic Acids Res       Date:  2020-07-02       Impact factor: 16.971

  1 in total

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