牙周膜细胞体外调控牙龈成纤维细胞表型。
Regulation of gingival fibroblast phenotype by periodontal ligament cells in vitro.
机构信息
Centre for Host-Microbiome Interactions, Faculty of Dentistry, Oral & Craniofacial Sciences, King's College London, London, UK.
Department of Periodontology, Faculty of Dentistry, Padjadjaran University, Bandung, Indonesia.
出版信息
J Periodontal Res. 2022 Apr;57(2):402-411. doi: 10.1111/jre.12971. Epub 2022 Jan 17.
OBJECTIVES
Stem cell transplantation has shown modest effects on periodontal tissue regeneration, and it is still unclear how regenerative effects utilizing this modality are mediated. A greater understanding of the basic interactions between implanted and host cells is needed to improve future strategies. The aims of this study were to investigate the effects of periodontal ligament (PDL) cells on expression of periodontal markers and alkaline phosphatase (ALP) activity of gingival fibroblasts (GF).
MATERIALS AND METHODS
Primary human PDL cells were co-cultured with primary GF cultures either by direct co-culture with subsequent FACS sorting or indirect co-culture using transwell cultures and PDL cell conditioned medium. Expression of periodontal markers, asporin, nestin, and periostin, was assessed by qPCR and immunofluorescence staining. Alkaline phosphatase (ALP) expression was assessed by qPCR, histochemical staining, and activity assessed by para-nitrophenol enzymatic assay. Single cultures of PDL cells and GF were used as controls. The role of Wnt signaling on ALP activity was assessed via Dkk1-mediated inhibition.
RESULTS
PDL cells significantly upregulated expression of PDL markers in GF with both direct and indirect co-culture methods when compared to controls (6.05 vs. 0.73 and 59.48 vs. 17.55 fold change of asporin expression). PDL/GF cell co-cultures significantly increased ALP activity in GF when compared with single GF cultures. Similar results were obtained when using conditioned medium isolated from PDL cell cultures. Dkk1 caused dose-dependent reduction in ALP activity of GF cultured in PDL cell conditioned medium.
CONCLUSIONS
PDL cells stimulate expression of periodontal markers and osteogenic capacity of gingival fibroblasts via paracrine signaling which can be partially inhibited with addition of the Wnt antagonist, Dkk1.Further studies are required to identify specific secreted factors responsible for this activity.
目的
干细胞移植对牙周组织再生显示出适度的效果,但仍不清楚如何利用这种方式介导再生效果。为了改善未来的策略,需要更深入地了解植入细胞和宿主细胞之间的基本相互作用。本研究的目的是研究牙周韧带(PDL)细胞对牙龈成纤维细胞(GF)牙周标志物表达和碱性磷酸酶(ALP)活性的影响。
材料和方法
将原代人 PDL 细胞与原代 GF 培养物直接共培养,随后通过 FACS 分选,或通过 Transwell 培养和 PDL 细胞条件培养基间接共培养。通过 qPCR 和免疫荧光染色评估牙周标志物,如无翅型 MMTV 整合位点家族成员 4(asporin)、巢蛋白(nestin)和骨膜蛋白(periostin)的表达。通过 qPCR、组织化学染色和对硝基苯酚酶测定法评估碱性磷酸酶(ALP)的表达。单独培养的 PDL 细胞和 GF 作为对照。通过 Dkk1 介导的抑制作用评估 Wnt 信号对 ALP 活性的作用。
结果
与对照相比,PDL 细胞通过直接和间接共培养方法显著上调 GF 中牙周标志物的表达(asporin 表达的 6.05 倍与 0.73 倍和 59.48 倍与 17.55 倍)。与单独的 GF 培养物相比,PDL/GF 细胞共培养物显著增加了 GF 中的 ALP 活性。使用从 PDL 细胞培养物中分离的条件培养基也得到了类似的结果。Dkk1 导致在 PDL 细胞条件培养基中培养的 GF 中的 ALP 活性呈剂量依赖性降低。
结论
PDL 细胞通过旁分泌信号刺激牙周标志物的表达和牙龈成纤维细胞的成骨能力,这种作用可以通过添加 Wnt 拮抗剂 Dkk1 部分抑制。需要进一步的研究来确定负责这种活性的特定分泌因子。
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