Please use this identifier to cite or link to this item: http://hdl.handle.net/11452/31550
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dc.contributor.authorBillur, Deniz-
dc.contributor.authorKızıl, Şule-
dc.contributor.authorAydın, Sevim-
dc.contributor.authorÜnlü, Ağahan-
dc.date.accessioned2023-03-14T08:21:27Z-
dc.date.available2023-03-14T08:21:27Z-
dc.date.issued2015-06-18-
dc.identifier.citationTaşkapılıoğlu, M. Ö. vd. (2016). "Targeting apoptosis through FOXP1, and N-cadherin with glatiramer acetate in chick embryos during neural tube development". Turkish Neurosurgery, 26(4), 586-594.tr_TR
dc.identifier.issn1019-5149-
dc.identifier.urihttps://doi.org/10.5137/1019-5149.JTN.14518-15.3-
dc.identifier.urihttp://www.turkishneurosurgery.org.tr/abstract.php?id=1726-
dc.identifier.urihttp://hdl.handle.net/11452/31550-
dc.description.abstractAIM: To demonstrate the effect of glatiramer acetate (GA) in chick embryos on neural tube (NT) development, and to explore its effects of FOXP1, apoptosis, and N-cadherin. MATERIAL and METHODS: One hundred fertile, specific pathogen free eggs were divided into 5 groups for this study. The eggshell was windowed specifically at 24 hours of incubation. The embryos in Group 1 (n=20) were treated with 10 mu l physiological saline; in Group 2 the embryos (n=20) were given 10 mu l GA (equal to daily human therapeutic dose); 20 mu l GA (equal to twice daily human therapeutic dose) was injected to embryos in Group 3 (n=20); in Group 4 and 5, 30 mu l and 40 mu l GA were administered to the embryos (n=20) (equal to x3 and x4 daily human therapeutic dose, respectively). Each egg was re-incubated for 24 hours more. Then, histological and immunohistochemical evaluation of the subjects were done. RESULTS: The embryos with NT defect showed FOXP1 expression without N-cadherin or staining with N-cadherin in another location in our study. We interpreted this result as GA leading to an NT closure defect by increasing FOXP expression. Moreover, we also showed the reverse relation between FOXP1 and N-cadherin at the immunohistochemical level for the first time. CONCLUSION: GA affects the spinal cord development through FOXP in the chick embryo model at high doses.en_US
dc.language.isoenen_US
dc.publisherTürk Nöroşirürji Derneğitr_TR
dc.rightsinfo:eu-repo/semantics/openAccessen_US
dc.rightsAtıf Gayri Ticari Türetilemez 4.0 Uluslararasıtr_TR
dc.rights.urihttp://creativecommons.org/licenses/by-nc-nd/4.0/*
dc.subjectNeurosciences & neurologyen_US
dc.subjectSurgeryen_US
dc.subjectChick embryoen_US
dc.subjectGlatiramer acetateen_US
dc.subjectFOXPen_US
dc.subjectN-Cadherinen_US
dc.subjectSpinal cord developmenten_US
dc.subjectTranscription factor foxp3en_US
dc.subjectB-cell lymphomaen_US
dc.subjectMultiple-sclerosisen_US
dc.subjectImmune-responsesen_US
dc.subjectPregnant-womenen_US
dc.subjectFork headen_US
dc.subjectT-cellsen_US
dc.subjectDefectsen_US
dc.subjectExpressionen_US
dc.subjectGenesen_US
dc.subject.meshAnimalsen_US
dc.subject.meshApoptosisen_US
dc.subject.meshCadherinsen_US
dc.subject.meshChick embryoen_US
dc.subject.meshChickensen_US
dc.subject.meshEmbryonic developmenten_US
dc.subject.meshForkhead transcription factorsen_US
dc.subject.meshGlatiramer acetateen_US
dc.subject.meshNeural tubeen_US
dc.subject.meshNeural tube defectsen_US
dc.subject.meshRepressor proteinsen_US
dc.titleTargeting apoptosis through FOXP1, and N-cadherin with glatiramer acetate in chick embryos during neural tube developmenten_US
dc.typeArticleen_US
dc.identifier.wos000381591600018tr_TR
dc.identifier.scopus2-s2.0-85021855641tr_TR
dc.relation.publicationcategoryMakale - Uluslararası Hakemli Dergitr_TR
dc.contributor.departmentUludağ Üniversitesi/Tıp Fakültesi/Nöroşirürji Anabilim Dalı.tr_TR
dc.contributor.departmentUludağ Üniversitesi/Tıp Fakültesi/Nöroloji Anabilim Dalı.tr_TR
dc.contributor.departmentUludağ Üniversitesi/Tıp Fakültesi/Biyoistatistik Anabilim Dalı.tr_TR
dc.contributor.orcid0000-0001-5472-9065tr_TR
dc.identifier.startpage586tr_TR
dc.identifier.endpage594tr_TR
dc.identifier.volume26tr_TR
dc.identifier.issue4tr_TR
dc.relation.journalTurkish Neurosurgeryen_US
dc.contributor.buuauthorTaşkapılıoğlu, M. Ozgur-
dc.contributor.buuauthorTaşkapılıoğlu, Özlem-
dc.contributor.buuauthorOcakoğlu, Gökhan-
dc.contributor.buuauthorBekar, Ahmet-
dc.contributor.researcheridHLG-6346-2023tr_TR
dc.contributor.researcheridAAK-6623-2020tr_TR
dc.contributor.researcheridABB-8161-2020tr_TR
dc.contributor.researcheridAAH-5180-2021tr_TR
dc.contributor.researcheridAAW-5254-2020tr_TR
dc.relation.collaborationYurt içitr_TR
dc.indexed.trdizinTrDizintr_TR
dc.identifier.pubmed27400107tr_TR
dc.subject.wosClinical neurologyen_US
dc.subject.wosSurgeryen_US
dc.indexed.wosSCIEen_US
dc.indexed.scopusScopusen_US
dc.indexed.pubmedPubMeden_US
dc.wos.quartileQ4en_US
dc.contributor.scopusid25936798300tr_TR
dc.contributor.scopusid23037226400tr_TR
dc.contributor.scopusid15832295800tr_TR
dc.contributor.scopusid6603677218tr_TR
dc.subject.scopusCadmium; Head Circumference; Eutheriaen_US
dc.subject.emtreeCadherinen_US
dc.subject.emtreeForkhead transcription factoren_US
dc.subject.emtreeFOXP1 protein, humanen_US
dc.subject.emtreeGlatirameren_US
dc.subject.emtreeRepressor proteinen_US
dc.subject.emtreeAnimalen_US
dc.subject.emtreeApoptosisen_US
dc.subject.emtreeBiosynthesisen_US
dc.subject.emtreeChemically induceden_US
dc.subject.emtreeChick embryoen_US
dc.subject.emtreeChickenen_US
dc.subject.emtreeDrug effectsen_US
dc.subject.emtreeEmbryo developmenten_US
dc.subject.emtreeEmbryologyen_US
dc.subject.emtreeMetabolismen_US
dc.subject.emtreeNeural tubeen_US
dc.subject.emtreeNeural tube defecten_US
dc.subject.emtreePathologyen_US
dc.subject.emtreePhysiologyen_US
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