Application of artificial endonucleases to the exocytotic mechanism of extracellular matrix proteins from periodontal ligament cells.

• Project/Area Number: 26462822
• Research Category: Grant-in-Aid for Scientific Research (C)
• Allocation Type: Multi-year Fund
• Section: 一般
• Research Field: Functional basic dentistry
• Research Institution: Health Sciences University of Hokkaido
• Principal Investigator: Takuma Taishin 北海道医療大学, 歯学部, 名誉教授 (40095336)
• Co-Investigator(Kenkyū-buntansha): 岡山 三紀 北海道医療大学, 歯学部, 助教 (30382500) ; 荒川 俊哉 北海道医療大学, 歯学部, 准教授 (40306254)
• Project Period (FY): 2014-04-01 – 2017-03-31
• Project Status: Completed (Fiscal Year 2016)
• Budget Amount: ¥5,070,000 (Direct Cost: ¥3,900,000、Indirect Cost: ¥1,170,000); Fiscal Year 2016: ¥1,040,000 (Direct Cost: ¥800,000、Indirect Cost: ¥240,000); Fiscal Year 2015: ¥1,820,000 (Direct Cost: ¥1,400,000、Indirect Cost: ¥420,000); Fiscal Year 2014: ¥2,210,000 (Direct Cost: ¥1,700,000、Indirect Cost: ¥510,000)
• Keywords: ゲノム編集 / SNARE / 構成的分泌 / CRISPR/Cas9 / SNAP23 / 歯根膜細胞 / HAP1細胞 / TALEN / 遺伝子ノックアウト / 人工ヌクレアーゼ / 遺伝子ノックアウト細胞 / HeLa細胞 / ハプロイド細胞

Outline of Final Research Achievements

In previous studies, constitutive exocytosis was normal in HeLa cells, whose SNAP23 was knocked down by up to 90% with its specific siRNAs, although SNAP23 null mice resulted in embryonic lethality at E3.5 before uterine implantation. To evaluate the role of SNAP23 in cell proliferation and constitutive exocytosis, we knocked out the gene by the application of CRISPR/Cas9 technology to HAP1 cells, a near haploid human cell line. The SNAP23-/ HAP1 cells had a 2-base pair-deletion in the SNAP23 gene; no SNAP23 protein was detectable by western blotting. The initial growth rate of the KO cell line was decreased by 40%, although the constitutive exocytosis of CLuc, a secreted luciferase of Cypridina noctiluca, and GFP-tagged human growth hormone was normal. The DNA microarray analysis showed that SNAP23 KO markedly influenced the expression of many genes. These results demonstrate that SNAP23 is not essential for cell proliferation or constitutive exocytosis.

Research Products

• [Presentation] SNAREタンパク質ノックアウトHAP1細胞の遺伝子発現比較解析． (2016)
  • Author(s): 荒川俊哉，岡山三紀，溝口到，田隈泰信
  • Organizer: 第89回日本生化学会大会
  • Place of Presentation: 仙台国際センター
  • Year and Date: 2016-09-25
• [Presentation] SNAREノックアウトHAP1細胞における遺伝子発現解析-SNAP23, Syntaxin4, Syntaxin2ノックアウトでの遺伝子発現比較． (2016)
  • Author(s): 荒川俊哉，岡山三紀，溝口到，田隈泰信
  • Organizer: 第58回歯科基礎医学会学術大会
  • Place of Presentation: 札幌コンベンションセンター
  • Year and Date: 2016-08-24
• [Presentation] CRISPR/Cas9法でSNAP23をKOした細胞の機構解析 (2015)
  • Author(s): 田隈泰信、荒川俊哉、岡山三紀、溝口到
  • Organizer: 第60回日本唾液腺学会学術集会
  • Place of Presentation: 文京学院大学本郷キャンパス
  • Year and Date: 2015-12-05
• [Presentation] SNAP23およびSyntaxin4ノックアウトHAP1細胞における遺伝子発現と細胞機能の解析 (2015)
  • Author(s): 荒川俊哉、岡山三紀、溝口到、田隈泰信
  • Organizer: 第88回日本生化学会大会
  • Place of Presentation: 神戸ポートアイランド
  • Year and Date: 2015-12-01
• [Presentation] SNAP23ノックアウトHAP1細胞の機能解析 (2015)
  • Author(s): 荒川俊哉、岡山三紀、溝口到、田隈泰信
  • Organizer: 第57回歯科基礎医学会学術大会
  • Place of Presentation: 新潟コンベンションセンター
  • Year and Date: 2015-09-11
• [Presentation] Is SNAP23 essential for constitutive exocytosis? (2015)
  • Author(s): Takuma T, Arakawa T, Okayama M, Mizoguchi I
  • Organizer: IADR (International Association for Dental Research)
  • Place of Presentation: アメリカ合衆国マサチューセッツ州ボストン､コンベンションセンター
  • Year and Date: 2015-03-11 – 2015-03-14