Tau protein kinase I converts normal tau protein into A68-like component of paired helical filaments.

  1. K Ishiguro,
  2. M Takamatsu,
  3. K Tomizawa,
  4. A Omori,
  5. M Takahashi,
  6. M Arioka,
  7. T Uchida and
  8. K Imahori
  1. Mitsubishi Kasei Institute of Life Sciences, Tokyo, Japan.

    Abstract

    From bovine brain microtubules we purified tau protein kinase I (TPKI, Mr 45,000 on sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) and tau protein kinase II (TPKII) whose activity was attributed to a 30-kDa protein on SDS-PAGE by affinity-labeling using an ATP analog. Both kinases were activated by tubulin. TPKII, but not TPKI, phosphorylated tau fragment peptides previously used for detection of a Ser/ThrPro kinase activity. Therefore, TPKII was considered to be the Ser/ThrPro kinase. TPKI was more effective than TPKII for producing the decrease of tau-1 immunoreactivity and mobility shift of tau on SDS-PAGE. Moreover, TPKI, but not TPKII nor other well-known protein kinases, generated an epitope present on paired helical filaments. These findings suggested that tau phosphorylated by TPKI resembled A-68, a component of paired helical filaments.

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    1. May 25, 1992 The Journal of Biological Chemistry, 267, 10897-10901.
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