@phdthesis{Wilhelm2018,
  author    = {Wilhelm, Christian},
  title     = {Die Rolle von Chronophin bei Schlaganfall-induziertem Funktionsverlust der Blut-Hirn-Schranke},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-163877},
  school      = {Universit{\"a}t W{\"u}rzburg},
  year      = {2018},
  abstract  = {Der isch{\"a}mische Schlaganfall ist mit einer j{\"a}hrlichen Inzidenz von 200/100 000 Einwohnern die h{\"a}ufigste Gef{\"a}ßerkrankung in Deutschland. Atherothrombose, arterielle Hypertonie und Embolien unterschiedlichen Ursprungs sind die wesentlichen Ursachen des isch{\"a}mischen Schlaganfalls. Die neurologischen Defizite nach einem Schlaganfall resultieren aus einem gest{\"o}rten zerebralen Blutfluss und somit einer insuffizienten Sauerstoffversorgung. Zus{\"a}tzlich ist die {\"O}dembildung, welche von einer gesteigerten Permeabilit{\"a}t der Blut-Hirn-Schranke verursacht wird, am neuronalen Zelltod beteiligt. Chronophin ist eine Aktinzytoskelett-regulierende Serin-Phosphatase. In einem isch{\"a}mischen Schlaganfall-Modell konnte im Rahmen dieser Arbeit gezeigt werden, dass der globale Verlust von Chronophin zu einer vermehrten {\"O}dembildung und einem aggravierten neurologischen Zustand der M{\"a}use im Vergleich zu wildtypischen Kontrollen f{\"u}hrte. Hirnlysate von wildtypischen M{\"a}usen zeigten verringerte Chronophin-Level in der vom Schlaganfall betroffenen Hemisph{\"a}re. Jedoch konnten initiale immunhistochemische und zellbiologische Untersuchungen weder Chronophin-abh{\"a}ngige Ver{\"a}nderungen der Blut-Hirn-Schranke feststellen noch einen zerebralen Zelltyp identifizieren, der f{\"u}r den sch{\"u}tzenden Effekt von Chronophin verantwortlich ist. Diese Ergebnisse weisen auf einen komplexen, vielzelligen Mechanismus hin, dem die sch{\"u}tzende Rolle von Chronophin im isch{\"a}mischen Schlaganfall unterliegt. Die Entschl{\"u}sselung dieses Mechanismus ist Aufgabe k{\"u}nftiger Untersuchungen.},
  subject      = {Schlaganfall},
  language  = {de}
}
@article{SchulzeHuttererSaboetal.2018,
  author    = {Schulze, Markus and Hutterer, Maria and Sabo, Anja and Hoja, Sabine and Lorenz, Julia and Rothhammer-Hampl, Tanja and Herold-Mende, Christel and Floßbach, Lucia and Monoranu, Camelia and Riemenschneider, Markus J.},
  title     = {Chronophin regulates active vitamin B6 levels and transcriptomic features of glioblastoma cell lines cultured under non-adherent, serum-free conditions},
  series = {BMC Cancer},
  volume    = {18},
  journal   = {BMC Cancer},
  doi       = {10.1186/s12885-018-4440-4},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-234645},
  year      = {2018},
  abstract  = {Background The phosphatase chronophin (CIN/PDXP) has been shown to be an important regulator of glioma cell migration and invasion. It has two known substrates: p-Ser3-cofilin, the phosphorylated form of the actin binding protein cofilin, and pyridoxal 5′-phosphate, the active form of vitamin B6. Phosphoregulation of cofilin, among other functions, plays an important role in cell migration, whereas active vitamin B6 is a cofactor for more than one hundred enzymatic reactions. The role of CIN has yet only been examined in glioblastoma cell line models derived under serum culture conditions. Results We found that CIN is highly expressed in cells cultured under non-adherent, serum-free conditions that are thought to better mimic the in vivo situation. Furthermore, the substrates of CIN, p-Ser3-cofilin and active vitamin B6, were significantly reduced as compared to cell lines cultured in serum-containing medium. To further examine its molecular role we stably knocked down the CIN protein with two different shRNA hairpins in the glioblastoma cell lines NCH421k and NCH644. Both cell lines did not show any significant alterations in proliferation but expression of differentiation markers (such as GFAP or TUBB3) was increased in the knockdown cell lines. In addition, colony formation was significantly impaired in NCH644. Of note, in both cell lines CIN knockdown increased active vitamin B6 levels with vitamin B6 being known to be important for S-adenosylmethionine biosynthesis. Nevertheless, global histone and DNA methylation remained unaltered as was chemoresistance towards temozolomide. To further elucidate the role of phosphocofilin in glioblastoma cells we applied inhibitors for ROCK1/2 and LIMK1/2 to our model. LIMK- and ROCK-inhibitor treatment alone was not toxic for glioblastoma cells. However, it had profound, but antagonistic effects in NCH421k and NCH644 under chemotherapy. Conclusion In non-adherent glioblastoma cell lines cultured in serum-free medium, chronophin knockdown induces phenotypic changes, e.g. in colony formation and transcription, but these are highly dependent on the cellular background. The same is true for phenotypes observed after treatment with inhibitors for kinases regulating cofilin phosphorylation (ROCKs and LIMKs). Targeting the cofilin phosphorylation pathway might therefore not be a straightforward therapeutic option in glioblastoma.},
  language  = {en}
}
@article{JeanclosKnoblochHoffmannetal.2020,
  author    = {Jeanclos, Elisabeth and Knobloch, Gunnar and Hoffmann, Axel and Fedorchenko, Oleg and Odersky, Andrea and Lamprecht, Anna-Karina and Schindelin, Hermann and Gohla, Antje},
  title     = {Ca\(^{2+}\) functions as a molecular switch that controls the mutually exclusive complex formation of pyridoxal phosphatase with CIB1 or calmodulin},
  series = {FEBS Letters},
  volume    = {594},
  journal   = {FEBS Letters},
  number    = {13},
  doi       = {10.1002/1873-3468.13795},
  url       = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-217963},
  pages     = {2099 -- 2115},
  year      = {2020},
  abstract  = {Pyridoxal 5′-phosphate (PLP) is an essential cofactor for neurotransmitter metabolism. Pyridoxal phosphatase (PDXP) deficiency in mice increases PLP and γ-aminobutyric acid levels in the brain, yet how PDXP is regulated is unclear. Here, we identify the Ca\(^{2+}\)- and integrin-binding protein 1 (CIB1) as a PDXP interactor by yeast two-hybrid screening and find a calmodulin (CaM)-binding motif that overlaps with the PDXP-CIB1 interaction site. Pulldown and crosslinking assays with purified proteins demonstrate that PDXP directly binds to CIB1 or CaM. CIB1 or CaM does not alter PDXP phosphatase activity. However, elevated Ca\(^{2+}\) concentrations promote CaM binding and, thereby, diminish CIB1 binding to PDXP, as both interactors bind in a mutually exclusive way. Hence, the PDXP-CIB1 complex may functionally differ from the PDXP-Ca\(^{2+}\)-CaM complex.},
  language  = {en}
}