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In-Vivo Application of Manganese-Labeled Immunocytes

https://repo.qst.go.jp/records/69618
https://repo.qst.go.jp/records/69618
7a02140b-e588-4f9c-a22b-f0dc82a8b000
Item type 会議発表用資料 / Presentation(1)
公開日 2008-12-02
タイトル
タイトル In-Vivo Application of Manganese-Labeled Immunocytes
言語
言語 eng
資源タイプ
資源タイプ識別子 http://purl.org/coar/resource_type/c_c94f
資源タイプ conference object
アクセス権
アクセス権 metadata only access
アクセス権URI http://purl.org/coar/access_right/c_14cb
著者 Odaka, Kenichi

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Odaka, Kenichi

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Aoki, Ichio

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Aoki, Ichio

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Moriya, Junji

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Moriya, Junji

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Tateno, Kaoru

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Tadokoro, Hiroyuki

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Minamino, Tohru

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Irie, Toshiaki

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Irie, Toshiaki

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Komuro, Issei

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Komuro, Issei

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Kanno, Iwao

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小高 謙一

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青木 伊知男

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森谷 純治

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舘野 馨

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田所 裕之

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入江 俊章

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菅野 巖

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抄録
内容記述タイプ Abstract
内容記述 Presentation Number 1034
\nIn-Vivo Application of Manganese-Labeled Immunocytes
\nKenichi Odaka1, Ichio Aoki1, Junji Moriya2, Kaoru Tateno2, Hiroyuki Tadokoro3, Tohru Minamino2, Toshiaki Irie1, Issei Komuro2, Kanno Iwao1, 1National Institute of Radiological Sciences, Japan; 2Chiba University, Japan; 3Tokai University, Japan. Contact e-mail: odaka@nirs.go.jp
\nOBJECTIVES: Recently, iron-oxide nanoparticles allows in-vivo trafficking of transplanted cells such as phagocyte and neural stem cell using magnetic resonance imaging (MRI). Although iron-oxide nanoparticles provide excellent sensitivity and contrast, it is difficult to label for non-phagocyte such as immunocyte due to size of the particle. On the other hand, although manganese (Mn) has poor sensitivity than the iron-oxide nanoparticles, Mn can provide positive contrast on T1-weighted MRI as a result of T1 (longitudinal relaxation time) shortening. In addition, most of cells are easily labeled by Mn because Mn2+ can pass the divalent calcium-ion channel. Therefore, we evaluated whether Mn-labeled cells can provide enough positive enhancement for cell tracking in-vitro and in-vivo. MATERIAL AND METHODS: Immunocytes of rat were separated from whole blood using centrifugation. Then they were incubated with MnCl2 for labeling. Ischemic models of the lower limbs were prepared 6 hours before cell injection in the rats. The labeled cells were topically injected into the ischemic left leg of the rats. Saline was also topically injected into the ischemic right leg as a control. MRI measurements were performed using 7.0 Tesla horizontal MRI immediately, 24 hours, and 48 hours after the injection. RESULTS: Immediately after the injection, both Mn-labeled cells and saline provide signal reduction on the T1-weighted MRI. At 48 hours after injection, Mn-labeled cells were detected as a double layered structure which has a positive outline and negative core, although injected saline was disappeared. Regeneration of blood flow was better in the immunocytes transplanted side than in the control. CONCLUSION: This study describes a novel contrast agent for transplanted immunocytes with the capability of the measurement of the transplanted area. In addition, it also can provide enough T1-positive MRI signal for tracing immunocytes and may be suitable for in-vivo trafficking of ischemic disease and regeneration researches.
\nDisclosure of author financial interest or relationships:
\nK. Odaka, Japan Cardiovascular Research Foundation, Grant/research support; I. Aoki, None; J. Moriya, None; K. Tateno, None; H. Tadokoro, None; T. Minamino, None; T. Irie, None; I. Komuro, None; K. Iwao, None.
会議概要(会議名, 開催地, 会期, 主催者等)
内容記述タイプ Other
内容記述 2008 World Molecular Imaging Congress
発表年月日
日付 2008-09-13
日付タイプ Issued
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