Five novel SLC7A7 variants and y+L gene-expression pattern in cultured lymphoblasts from Japanese patients with lysinuric protein intolerance

Yutaka Shoji*, Atsuko Noguchi, Yasuko Shoji*, Mika Matsumori, Yuhei Takasago, Masaki Takayanagi, Yoshihiro Yoshida, Kenji Ihara, Toshiro Hara, Shuichi Yamaguchi, Makoto Yoshino, Masayuki Kaji, Shigenori Yamamoto, Akio Nakai, Akio Koizumi, Youichi Hokezu, Keiji Nagamatsu, Hitoshi Mikami, Isao Kitajima, Goro Takada

*この論文の責任著者

研究成果: ジャーナルへの寄稿学術論文査読

22 被引用数 (Scopus)

抄録

Two distinct human light subunits of the heteromeric amino acid transporter, y+LAT-1 coded by SLC7A7 and y+LAT-2 coded by SLC7A6, are both known to induce transport system y+L activity. SLC7A7 has already been identified as the gene responsible for lysinuric protein intolerance (LPI). We successfully identified five novel SLC7A7 variants (S238F, S489P, 1630delC, 1673delG, and IVS3-IVSSdel9.7kb) in Japanese patients with LPI by PCR amplification and direct DNA sequencing. In addition, we performed a semi-quantitative expression analysis of SLC7A7 and SLC7A6 in human tissue. In normal tissue, the gene-expression ratio of SLC7A6 to SLC7A7 was high in the brain, muscle, and cultured skin fibroblasts; low in the kidneys and small intestine; and at an intermediate level in peripheral blood leukocytes, the lungs, and cultured lymphoblasts. The gene-expression ratio of SLC7A6 to SLC7A7 in cultured lymphoblasts was significantly different between normal subjects and LPI patients with R410X and/or S238F, where the relative amount of SLC7A7 mRNA was significantly lower and the relative amount of SLC7A6 mRNA was statistically higher in affected lymphoblasts than in normal cells. Expression of SLC7A7 and SLC7A6 may thus be interrelated in cultured lymphoblasts.

本文言語英語
ページ(範囲)375-381
ページ数7
ジャーナルHuman Mutation
20
5
DOI
出版ステータス出版済み - 2002

ASJC Scopus 主題領域

  • 遺伝学
  • 遺伝学(臨床)

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