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Dive into the research topics where Andrew Slatter is active.

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Featured researches published by Andrew Slatter.


Genes, Chromosomes and Cancer | 2014

Clinical and pathological impact of VHL, PBRM1, BAP1, SETD2, KDM6A, and JARID1c in clear cell renal cell carcinoma

Lucy Gossage; Muhammed Murtaza; Andrew Slatter; Conrad Lichtenstein; Anne Warren; Beverley Haynes; Francesco Marass; Ian Roberts; Susan J. Shanahan; Andreas Claas; Andrew Dunham; Andrew May; Nitzan Rosenfeld; Tim Forshew; Tim Eisen

VHL is mutated in the majority of patients with clear cell renal cell carcinoma (ccRCC), with conflicting clinical relevance. Recent studies have identified recurrent mutations in histone modifying and chromatin remodeling genes, including BAP1, PBRM1, SETD2, KDM6A, and JARID1c. Current evidence suggests that BAP1 mutations are associated with aggressive disease. The clinical significance of the remaining genes is unknown. In this study, targeted sequencing of VHL and JARID1c (entire genes) and coding regions of BAP1, PBRM1, SETD2, and KDM6A was performed on 132 ccRCCs and matched normal tissues. Associations between mutations and clinical and pathological outcomes were interrogated. Inactivation of VHL (coding mutation or promoter methylation) was seen in 75% of ccRCCs. Somatic noncoding VHL alterations were identified in 29% of ccRCCs and may be associated with improved overall survival. BAP1 (11%), PBRM1 (33%), SETD2 (16%), JARID1c (4%), and KDM6A (3%) mutations were identified. BAP1‐mutated tumors were associated with metastatic disease at presentation (P = 0.023), advanced clinical stage (P = 0.042) and a trend towards shorter recurrence free survival (P = 0.059) when compared with tumors exclusively mutated for PBRM1. Our results support those of recent publications pointing towards a role for BAP1 and PBRM1 mutations in risk stratifying ccRCCs. Further investigation of noncoding alterations in VHL is warranted.


Nucleic Acids Research | 2013

Reflex: intramolecular barcoding of long-range PCR products for sequencing multiple pooled DNAs

James Casbon; Andrew Slatter; Esther Musgrave-Brown; Robert Osborne; Conrad Lichtenstein; Sydney Brenner

We present an intramolecular reaction, Reflex™, to derive shorter, sequencer-ready, daughter polymerase chain reaction products from a pooled population of barcoded long-range polymerase chain reaction products, whilst still preserving the cognate DNA barcodes. Our Reflex workflow needs only a small number of primer extension steps to rapidly enable uniform sequence coverage of long contiguous sequence targets in large numbers of samples at low cost on desktop next-generation sequencers.


Archive | 2010

Compositions and Methods for Intramolecular Nucleic Acid Rearrangement

Sydney Brenner; Gi Mikawa; Robert Osborne; Andrew Slatter


Archive | 2011

Methods and compositions for polynucleotide library production, immortalization and region of interest extraction

Robert Osborne; Andrew Slatter


Archive | 2010

Sorting asymmetrically tagged nucleic acids by selective primer extension

Esther Musgrave-Brown; Gi Mikawa; Robert Osborne; Andrew Slatter


Archive | 2011

Region of Interest Extraction and Normalization Methods

Robert Osborne; Andrew Slatter


Archive | 2017

METHODS FOR ANALYZING NUCLEIC ACIDS FROM SINGLE CELLS

Sydney Brenner; Gi Mikawa; Robert Osborne; Andrew Slatter


Archive | 2013

Compositions et procédés pour le réarrangement intramoléculaire d'acide nucléique

Robert Osborne; Andrew Slatter; James Casbon


BMC Proceedings | 2012

Reflex™: a novel method to sequence barcoded long-range PCR products in a pooled population of hundreds of DNA samples

James Casbon; Andrew Slatter; Esther Musgrave-Brown; Robert Osborne; Conrad Lichtenstein; Sydney Brenner


Archive | 2011

Methods for replicating polynucleotides with secondary structure

Sydney Brenner; Robert Osborne; Andrew Slatter

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James Casbon

University of Cambridge

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Anne Warren

Cambridge University Hospitals NHS Foundation Trust

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Ian Roberts

University of Cambridge

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