Kumi Nagao scite author profile

Kumi Nagao

5Publications

179Citation Statements Received

44Citation Statements Given

How they've been cited

201

171

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Affiliations

Doshisha University, HistoGenetics (United States), Tokyo Medical University

Publications

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Expression Profile of a γ-Deletion Variant of the Human Telomerase Reverse Transcriptase Gene

Higuchi¹,

Ohyashiki

et al. 2003

Neoplasia

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The human telomerase reverse transcriptase (hTERT) is an essential component of the holoenzyme complex that adds telomeric repeats to the ends of chromosomes. The hTERT transcript has been shown to have two deletion type alternative splicing sites. One deletion site induces the alpha-deletion variant, lacking 36 bp from exon 6, and the other induces the beta-deletion variant, lacking 182 bp from exons 7 and 8. Here, we identified a novel deletion variant of the hTERT transcript in hepatocellular carcinoma cell lines. The deleted transcript was characterized by an in-frame deletion of 189 bp, spanning nucleotides 2710 to 2898, corresponding to the complete loss of exon 11 (gamma-deletion). The region lacking in the gamma-deletion lies within RT motifs D and E, suggesting that it is missing conserved residues from the catalytic core of the protein. Both gamma- and alpha-deletion variants were occasionally detected, but the beta-deletion variant was frequently observed. Our results may provide important information for more detailed studies on the regulation of telomerase activity.

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Levels of telomerase catalytic subunit mRNA as a predictor of potential malignancy.

Higuchi¹,

Nagao²,

Kanamaru³

et al. 1999

Int J Oncol

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Quantification of telomerase activity in human liver tissues by fluorescence-based TRAP analysis

Higuchi¹,

Nagao²,

Komatsu

1997

Hepatology Research

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Identification of an alternative splicing transcript for the resistin gene and distribution of its mRNA in human tissue

Nohira

Nagao

Kameyama³

et al. 2004

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Objective: Adipocytes secrete a number of molecules such as tumor necrosis factor-alpha, leptin and free fatty acids that can influence the ability of the body to metabolize glucose. Recently, a novel 12.5 kDa cysteine-rich protein, termed resistin, was shown to be secreted by adipocytes. Resistin expression was markedly induced during the conversion of 3T3-L1 cells to mature adipocytes. Expression of resistin has been studied in human, mouse and rat; however, sequence information about an alternative splicing variant (ASV) of resistin mRNA has not been reported. In the present study, we investigated the occurrence of a novel ASV of the resistin gene in human normal tissues. Design and methods: We identified a novel ASV of resistin mRNA in human lung tissue by RT-PCR analysis in human lung tissue. We then investigated a novel ASV of resistin mRNA by real-time PCR analysis in 26 different types of normal human tissues. Results and conclusions: We identified a novel deletion variant of the resistin transcript in the normal human tissues. The deleted transcript of resistin was characterized by an in-frame deletion of 78 bp, corresponding to the complete loss of exon 2 (resistin delta2 ASV). Thus, resistin delta2 ASV causes protein truncation. Our results provide the basis for more detailed studies on the regulation of resistin activity, and should assist in the development of clinical trials with resistin for the central regulation of adipogenesis and adipocyte metabolism.

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Quantitative relationship between functionally active telomerase and major telomerase components (hTERT and hTR) in acute leukaemia cells

Ohyashiki

Higuchi²,

Nagao³

et al. 2005

Br J Cancer

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Functionally active telomerase is affected at various steps including transcriptional and post-transcriptional levels of major telomerase components (hTR and human telomerase reverse transcriptase (hTERT)). We therefore developed a rapid and sensitive method to quantify hTERT and its splicing variants as well as the hTR by a Taqman real-time reverse transcriptase -polymerase chain reaction to determine whether their altered expression may contribute to telomere attrition in vivo or not. Fresh leukaemia cells obtained from 38 consecutive patients were used in this study. The enzymatic level of telomerase activity measured by TRAP assay was generally associated with the copy numbers of full-length hTERT þ a þ b mRNA (P ¼ 0.0024), but did not correlate with hTR expression (P ¼ 0.6753). In spite of high copy numbers of full-length hTERT mRNA, telomerase activity was low in some cases correlating with low copy numbers of hTR, raising the possibility that alteration of the hTR : hTERT ratio may affect functionally active telomerase activity in vivo. The spliced nonactive hTERT mRNA tends to be lower in patients with high telomerase activity, suggesting that this epiphenomenon may play some role in telomerase regulation. An understanding of the complexities of telomerase gene regulation in biologically heterogeneous leukaemia cells may offer new therapeutic approaches to the treatment of acute leukaemia.

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Kumi Nagao

Expression Profile of a γ-Deletion Variant of the Human Telomerase Reverse Transcriptase Gene

Levels of telomerase catalytic subunit mRNA as a predictor of potential malignancy.

Quantification of telomerase activity in human liver tissues by fluorescence-based TRAP analysis

Identification of an alternative splicing transcript for the resistin gene and distribution of its mRNA in human tissue

Quantitative relationship between functionally active telomerase and major telomerase components (hTERT and hTR) in acute leukaemia cells

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