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Dive into the research topics where Molly He is active.

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Featured researches published by Molly He.


Genome Biology | 2016

Characterization of chromatin accessibility with a transposome hypersensitive sites sequencing (THS-seq) assay

Brandon C. Sos; Ho-Lim Fung; Derek Gao; Trina Faye Osothprarop; Amirali Kia; Molly He; Kun Zhang

Chromatin accessibility captures in vivo protein-chromosome binding status, and is considered an informative proxy for protein-DNA interactions. DNase I and Tn5 transposase assays require thousands to millions of fresh cells for comprehensive chromatin mapping. Applying Tn5 tagmentation to hundreds of cells results in sparse chromatin maps. We present a transposome hypersensitive sites sequencing assay for highly sensitive characterization of chromatin accessibility. Linear amplification of accessible DNA ends with in vitro transcription, coupled with an engineered Tn5 super-mutant, demonstrates improved sensitivity on limited input materials, and accessibility of small regions near distal enhancers, compared with ATAC-seq.


Nature Communications | 2015

DNA sequencing using polymerase substrate-binding kinetics

Michael Previte; Chunhong Zhou; Matthew William Kellinger; Rigo Pantoja; Cheng-Yao Chen; Jin Shi; Amirali Kia; Sergey Etchin; John S. Vieceli; Ali Nikoomanzar; Erin Bomati; Christian Gloeckner; Mostafa Ronaghi; Molly He

Next-generation sequencing (NGS) has transformed genomic research by decreasing the cost of sequencing. However, whole-genome sequencing is still costly and complex for diagnostics purposes. In the clinical space, targeted sequencing has the advantage of allowing researchers to focus on specific genes of interest. Routine clinical use of targeted NGS mandates inexpensive instruments, fast turnaround time and an integrated and robust workflow. Here we demonstrate a version of the Sequencing by Synthesis (SBS) chemistry that potentially can become a preferred targeted sequencing method in the clinical space. This sequencing chemistry uses natural nucleotides and is based on real-time recording of the differential polymerase/DNA-binding kinetics in the presence of correct or mismatch nucleotides. This ensemble SBS chemistry has been implemented on an existing Illumina sequencing platform with integrated cluster amplification. We discuss the advantages of this sequencing chemistry for targeted sequencing as well as its limitations for other applications.


Frontiers in Plant Science | 2018

Sequencing and Analysis of Strobilanthes cusia (Nees) Kuntze Chloroplast Genome Revealed the Rare Simultaneous Contraction and Expansion of the Inverted Repeat Region in Angiosperm

Haimei Chen; Junjie Shao; Hui Zhang; Mei Jiang; Linfang Huang; Zhao Zhang; Dan Yang; Molly He; Mostafa Ronaghi; Xi Luo; Botao Sun; Wuwei Wu; Chang Liu

Ban-Lan-Gen, the root tissues derived from several morphologically indistinguishable plant species, have been used widely in traditional Chinese medicines for numerous years. The identification of reliable markers to distinguish various source plant species is critical for the effective and safe use of products containing Ban-Lan-Gen. Here, we analyzed and characterized the complete chloroplast (cp) genome sequence of Strobilanthes cusia (Nees) Kuntze to identify high-resolution markers for the species determination of Southern Ban-Lan-Gen. Total DNA was extracted and subjected to next-generation sequencing. The cp genome was then assembled, and the gaps were filled using PCR amplification and Sanger sequencing. Genome annotation was conducted using CpGAVAS web server. The genome was 144,133 bp in length, presenting a typical quadripartite structure of large (LSC; 91,666 bp) and small (SSC; 17,328 bp) single-copy regions separated by a pair of inverted repeats (IRs; 17,811 bp). The genome encodes 113 unique genes, including 79 protein-coding, 30 transfer RNA, and 4 ribosomal RNA genes. A total of 20 tandem, 2 forward, and 6 palindromic repeats were detected in the genome. A phylogenetic analysis based on 65 protein-coding genes showed that S. cusia was closely related to Andrographis paniculata and Ruellia breedlovei, which belong to the same family, Acanthaceae. One interesting feature is that the IR regions apparently undergo simultaneous contraction and expansion, resulting in the presence of single copies of rps19, rpl2, rpl23, and ycf2 in the LSC region and the duplication of psbA and trnH genes in the IRs. This study provides the first complete cp genome in the genus Strobilanthes, containing critical information for the classification of various Strobilanthes species in the future. This study also provides the foundation for precisely determining the plant sources of Ban-Lan-Gen.


Archive | 2011

Conformational probes and methods for sequencing nucleic acids

Molly He; Cheng-Yao Chen; Eric Kool; Mostafa Ronaghi; Michael Previte; Rigo Pantoja


Archive | 2012

Apparatus and methods for kinetic analysis and determination of nucleic acid sequences

Michael Previte; Molly He; Rigo Pantoja; Cheng-Yao Chen; Chunhong Zhou


Archive | 2017

Contiguity preserving transposition

Frank J. Steemers; Kevin L. Gunderson; Fan Zhang; Jason Richard Betley; Niall Anthony Gormley; Wouter Meuleman; Jacqueline C. Weir; Avgousta Ioannou; Gareth Jenkins; Rosamond Jackson; Natalie Morrell; Dmitry K. Pokholok; Steven J Norberg; Molly He; Amirali Kia; Igor Goryshin; Rigo Pantoja


Archive | 2015

NUCLEIC ACID SYNTHESIS TECHNIQUES

Mostafa Ronaghi; Molly He; Cheng-Yao Chen; Michael Previte; Shane M. Bowen


Archive | 2015

MODIFIED TRANSPOSASES FOR IMPROVED INSERTION SEQUENCE BIAS AND INCREASED DNA INPUT TOLERANCE

Christian Gloeckner; Amirali Kia; Erin Bomati; Molly He; Haiying Li Grunenwald; Scott Kuersten; Trina Faye Osothprarop; Darin Haskins; Joshua Burgess; Anupama Khanna; Daniel Schlingman; Ramesh Vaidyanathan


BMC Biotechnology | 2017

Improved genome sequencing using an engineered transposase

Amirali Kia; Christian Gloeckner; Trina Faye Osothprarop; Niall Anthony Gormley; Erin Bomati; Michelle Stephenson; Igor Goryshin; Molly He


Archive | 2014

METHODS AND COMPOSITIONS FOR TARGETED NUCLEIC ACID SEQUENCING

Rigo Pantoja; Marie Hu; Erin Bomati; Molly He

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