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Featured researches published by J.R. Lee.


The EMBO Journal | 2002

MicroRNA maturation: stepwise processing and subcellular localization.

Yoontae Lee; Kipyoung Jeon; J.R. Lee; Sunyoung Kim; V. Narry Kim

MicroRNAs (miRNAs) constitute a novel, phylogenetically extensive family of small RNAs (∼22 nucleotides) with potential roles in gene regulation. Apart from the finding that miRNAs are produced by Dicer from the precursors of ∼70 nucleotides (pre‐miRNAs), little is known about miRNA biogenesis. Some miRNA genes have been found in close conjunction, suggesting that they are expressed as single transcriptional units. Here, we present in vivo and in vitro evidence that these clustered miRNAs are expressed polycistronically and are processed through at least two sequential steps: (i) generation of the ∼70 nucleotide pre‐miRNAs from the longer transcripts (termed pri‐miRNAs); and (ii) processing of pre‐miRNAs into mature miRNAs. Subcellular localization studies showed that the first and second steps are compartmentalized into the nucleus and cytoplasm, respectively, and that the pre‐miRNA serves as the substrate for nuclear export. Our study suggests that the regulation of miRNA expression may occur at multiple levels, including the two processing steps and the nuclear export step. These data will provide a framework for further studies on miRNA biogenesis.


Gene Therapy | 2003

Construction of a retroviral vector production system with the minimum possibility of a homologous recombination

Seung Shin Yu; Eunyoung Han; Youngtae Hong; J.R. Lee; Sujeong Kim; Sunyoung Kim

A recombination between the short homologous regions of nucleotide sequences in the retroviral vector and packaging cell line has been thought to be a major cause of the production of replication-competent retrovirus (RCR). Therefore, the removal of overlapping sequences between the vector and the packaging constructs is crucial for minimizing the possibility of homologous recombination, and therefore, the production of RCR. We have recently constructed a series of retroviral vectors that contain no viral coding sequences, but still produce high viral titer and high-level gene expression. However, many previously constructed murine leukemia viurs (MLV)-based packaging constructs contained significantly long 5′ and/or 3′ untranslated regions of MLV, which are also present in the retroviral vector, and as such could possibly lead to homologous recombination. To make a retroviral production system that is free from homologous recombination, we constructed expression plasmids for gag-pol and env, precisely starting from the start codon and ending at the stop codon of respective open reading frames. When the packaging function was provided from one plasmid, a vector containing bits of all three viral coding sequences produced RCR at a significant frequency, while our vector remained free of any RCR. Our retrovirus production system is anticipated to have the minimum possible frequency of RCR production due to the elimination of potential sites for homologous recombination. Based on these results, a highly efficient new packaging line Vamp that contains no overlapping sequences with our retroviral vector was also developed.


Journal of Gene Medicine | 2008

Development of an in vitro cell culture assay system for measuring the activation of a neighbouring gene by the retroviral vector.

Youngtae Hong; Seung Shin Yu; Nam-Kyung Yoon; Sung June Kang; J.R. Lee; Sujeong Kim; Jong-Mook Kim; Karim Lee; Jiwon Jang; Sunyoung Kim

The use of retroviral vectors has shown an actual clinical benefit in a few inherited diseases. However, the occurrence of cases of leukemia after the X‐SCID gene therapy trial raised concerns about the safety of insertional mutagenesis inherent to the biology of the retrovirus. Although the retrovirus has long been known to integrate into the host chromosome, and thus have the potential to activate the nearby gene, there has been no convenient method of studying or assaying such a cis‐activation phenomenon.


Molecular Therapy | 2007

Control of splicing efficiency by the mouse histone H2a element in a murine leukemia virus-based retroviral vector.

J.R. Lee; Seung Shin Yu; V. Narry Kim; Sunyoung Kim


Archive | 2007

Expression Vectors with Improved Safety

Sunyoung Kim; Sujeong Kim; J.R. Lee


Fertility and Sterility | 2008

Comparative study of two cryopreservation methods of human spermatozoa: vitrification versus slow freezing

Hye Jin Chang; J.R. Lee; Soo Jin Chae; B.C. Jee; Chang-Suk Suh; S. Kim


Fertility and Sterility | 2014

The effect of embryo transfer day oxytocin antagonist infusion on IVF outcomes: a systematic review and meta-analysis

Myo Sun Kim; Seul Ki Kim; J.R. Lee; B.C. Jee; Chang-Suk Suh; Hyunmin Choi; S. Kim


Fertility and Sterility | 2014

The effect of age and serum anti-müllerian hormone (AMH) level on fertilization rate (FR) in women with polycystic ovary syndrome (PCOS) after assisted reproductive technology (ART)

E. Lee; H. Kim; J.R. Lee; B.C. Jee; Seung-Yup Ku; Chang-Suk Suh; S. Kim; Y.M. Choi; Jun-Ran Kim


Fertility and Sterility | 2014

Effect of three different types of antifreeze proteins supplementation on mouse ovarian tissue vitrification and transplantation

Jung Jae Lee; Hyewon Youm; J.R. Lee; B.C. Jee; Chang-Suk Suh; Hyonkwang Choi; S. Kim


Fertility and Sterility | 2013

The association between menstrual history and parameters of healthcare screening test in postmenopausal women of Korean community

Kyoung Yong Moon; H. Kim; J.R. Lee; B.C. Jee; Chang-Suk Suh; S. Kim

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Chang-Suk Suh

Seoul National University

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S. Kim

Seoul National University

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B.C. Jee

Seoul National University

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Sunyoung Kim

Seoul National University

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Sujeong Kim

Seoul National University

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Seung Shin Yu

Seoul National University

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S.Y. Moon

Seoul National University

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V. Narry Kim

Seoul National University

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Y.M. Choi

Seoul National University

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Youngtae Hong

Seoul National University

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