Literature DB >> 25183780

From deep sequencing to actual clones.

Sara D'Angelo1, Sandeep Kumar2, Leslie Naranjo3, Fortunato Ferrara4, Csaba Kiss3, Andrew R M Bradbury5.   

Abstract

The application of deep sequencing to in vitro display technologies has been invaluable for the straightforward analysis of enriched clones. After sequencing in vitro selected populations, clones are binned into identical or similar groups and ordered by abundance, allowing identification of those that are most enriched. However, the greatest strength of deep sequencing is also its greatest weakness: clones are easily identified by their DNA sequences, but are not physically available for testing without a laborious multistep process involving several rounds of polymerization chain reaction (PCR), assembly and cloning. Here, using the isolation of antibody genes from a phage and yeast display selection as an example, we show the power of a rapid and simple inverse PCR-based method to easily isolate clones identified by deep sequencing. Once primers have been received, clone isolation can be carried out in a single day, rather than two days. Furthermore the reduced number of PCRs required will reduce PCR mutations correspondingly. We have observed a 100% success rate in amplifying clones with an abundance as low as 0.5% in a polyclonal population. This approach allows us to obtain full-length clones even when an incomplete sequence is available, and greatly simplifies the subcloning process. Moreover, rarer, but functional clones missed by traditional screening can be easily isolated using this method, and the approach can be extended to any selected library (scFv, cDNA, libraries based on scaffold proteins) where a unique sequence signature for the desired clones of interest is available.
© The Author 2014. Published by Oxford University Press. All rights reserved. For Permissions, please e-mail: journals.permissions@oup.com.

Entities:  

Keywords:  antibody; deep sequencing; inverse PCR; phage display; yeast display

Mesh:

Substances:

Year:  2014        PMID: 25183780      PMCID: PMC4191444          DOI: 10.1093/protein/gzu032

Source DB:  PubMed          Journal:  Protein Eng Des Sel        ISSN: 1741-0126            Impact factor:   1.650


  26 in total

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4.  In vitro display technologies reveal novel biopharmaceutics.

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5.  Conformations of the third hypervariable region in the VH domain of immunoglobulins.

Authors:  V Morea; A Tramontano; M Rustici; C Chothia; A M Lesk
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7.  Rapid interactome profiling by massive sequencing.

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8.  Precise determination of the diversity of a combinatorial antibody library gives insight into the human immunoglobulin repertoire.

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9.  Rapid and efficient cDNA library screening by self-ligation of inverse PCR products (SLIP).

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Review 2.  Integrating high-throughput screening and sequencing for monoclonal antibody discovery and engineering.

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Journal:  Immunology       Date:  2017-10-30       Impact factor: 7.397

3.  Selection of phage-displayed accessible recombinant targeted antibodies (SPARTA): methodology and applications.

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4.  High-Throughput Generation of In Silico Derived Synthetic Antibodies via One-step Enzymatic DNA Assembly of Fragments.

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5.  Proteome-wide Identification of Novel Ceramide-binding Proteins by Yeast Surface cDNA Display and Deep Sequencing.

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Review 7.  Deep sequencing in library selection projects: what insight does it bring?

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8.  Pacific Biosciences Sequencing and IMGT/HighV-QUEST Analysis of Full-Length Single Chain Fragment Variable from an In Vivo Selected Phage-Display Combinatorial Library.

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9.  A Simple Whole-Plasmid PCR Method to Construct High-Diversity Synthetic Phage Display Libraries.

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10.  One-Step Recovery of scFv Clones from High-Throughput Sequencing-Based Screening of Phage Display Libraries Challenged to Cells Expressing Native Claudin-1.

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