EFFECTS OF TRANSFORMING GROWTH FACTOR β AND RECOMBINANT HUMAN BONE MORPHOGENETIC PROTEIN 2 ON HUMAN PERIODONTAL LIGAMENT FIBROBLASTS

Objective To evaluate the effects of transforming growth factor β(TGF-β) and recombinant human bone morphogenetic protein 2 (rhBMP2) on human periodontal ligament fibroblasts (HPDLFs). Methods HPDLFs were done primary culture to detect the distinct concentrations of TGF-P and rhBMF2 on its proliferation, alkaline phosphatase (ALP) activity, osteocalcin (OC) synthesis and formation of the minerali-zed nodules, respectively. Results TGF-β (5～100ng/ml) significantly stimulated the proliferation of HPDLFs. The ALP activity of HPDLFs was evaluated evidently by 5ng/ml TGF-β. TGF-β( 0. 5 ～ 100ng/ml) had no effects on OC synthesis and formation of the mineralized nodules of HPDLFs. rhBMP2 (0. 25～2mg/ ml) had no remarkable effect on the proliferation of HPDLFs. The ALP activity, OC synthesis and forma-tion of the mineralized nodules of HPDLFs were significantly stimulated by 0. 5～ 2mg /ml rhBMP2. Conclusion The effects of TGF-β and rhBMP2 on HPDLFs are dose-dependent. TGF-P can stimulate HPDLFs to express the early marker of osteoblastic phenotype, and it lacks the ability to promote maturation of the osteogenic phenotype. rhBMP2 can not only stimulate the expression but also promote the maturation of osteoblas-tic phenotype of HPDLFs.

Relationship between diabetes and periodontal infection

Periodontal disease is a high prevalent disease.In the United States 47.2% of adults ≥ 30 years old have been diagnosed with some type of periodontitis.Longitudinal studies have demonstrated a two-way relationship between diabetes and periodontitis,with more severe periodontal tissue destruction in diabetic patients and poorer glycemic control in diabetic subjects with periodontal disease.Periodontal treatment can be successful in diabetic patients.Short term effects of periodontal treatment are similar in diabetic patients and healthy population but,more recurrence of periodontal disease can be expected in no well controlled diabetic individuals.However,effects of periodontitis and its treatment on diabetes metabolic control are not clearly defined and results of the studies remain controversial.

Elevated levels of inflammatory cytokines and high-sensitivity C-reactive protein in periodontitis patients in Kosovo: A pilot study

The following article has been retracted due to the investigation of complaints received against it. The Editorial Board found that the same contents have been published in another journal at the same time. The scientific community takes a very strong view on this matter, and the Open Journal of Stomatology treats all unethical behavior such as plagiarism seriously. This paper published in Vol.3 No.1 32-38, 2013 has been removed from this site. Title: Elevated levels of inflammatory cytokines and high-sensitivity C-reactive protein in periodontitis patients in Kosovo: A pilot study Authors: Zana Sllamniku-Dalipi, Hasan Mehmeti, Fatmir Dragidella, Ferit Kocani, Metush Disha, Kastriot Meqa, Luljeta Begolli, Gramos

Triclosan inhibits the activation of human periodontal ligament fibroblasts induced by lipopolysaccharide from Porphyromonas gingivalis

Periodontitis is a highly prevalent,chronic,non-specific,and immunologically devastating disease of periodontal tissues,caused by microbial infection.This study aims to examine the efficacy and protective mechanism of triclosan(TCS),a bisphenolic,non-cationic component of oral care products,against periodontal inflammation induced by lipopolysaccharide purified from Porphyromonas gingivalis(LPS-PG).TCS markedly downregulated interleukin-6(IL-6),IL-8,and IL-15 in human periodontal ligament fibroblasts(HPDLFs)treated with LPS-PG.By using a liquid chromatography-tandem mass spectrometry(LC-MS/MS)approach,318 differentially expressed proteins(161 upregulated and 157 downregulated)were identified in TCS-pretreated HPDLFs.TCS upregulated HSPA5 and HSP90B1 but downregulated HSPA2.Besides,TCS upregulated miR-548i in HPDLFs,which downregulated IL-15.These results indicate that TCS attenuates the activation of HPDLFs and downregulates the inflammatory cytokines through various mechanisms,thus highlighting its protective role in periodontal inflammation.

Influence of periodontitis and nonsurgical periodontal intervention on atherosclerosis diseases

Objective: Periodontitis and atherosclerosis diseases are chronic inflammatory disorders which are highly prevalent in populations. Nonsurgical periodontal intervention belongs to the initial therapy strategy to periodontal diseases. Periodontal pathogen can enter into blood stream through the ulceration epithelial resulting in bacteraemia when periodontitis is severe. The objective is to investigate the relationship between periodontitis and atherosclerosis diseases, and the influence of nonsurgical periodontal intervention on atheroma and atherosclerosis diseases. Methods: This study reviewed and analyzed the papers which published in the world associated with periodontitis or periodontal intervention on atherosclerosis diseases. Results: Periodontitis and periodontal infectious are important risk factors for atherosclerotic diseases. Much evidence has proved the durative severe periodontitis can result in bacteraemia and systemic inflammation, elevated C-response protein in serum, gingival microcirculation changed, periodontal microorganism reproduced, and endothelial dys-function and endocarditis. Nonsurgical periodontal intervention can remove the pathogenesis bacteria and calculus to recover periodontal health. Effective periodontal therapy can reduce bacteraemia and stop the hurt to vessels. Nonsurgical periodontal therapy may interfere periodontal bacteria, inhibit inflammation response and C-response protein, improving gingival microcirculation and vessel epithelial function to prevent atherosclerosis. Conclusion: Nonsurgical periodontal intervention can improve or decrease the rate of atherosclerotic disease by interfere the severe periodontitis. The detailed mechanism of periodontal intervention on atheroma and atherosclerotic disease is still need to be explored.

Immune Responses to HSP65/60 in Periodontal Disease

Chronic periodontitis (CP) is a chronic inflammatory condition which destroys the supporting tissues of teeth and increases in prevalence with age. Immune responses against heat shock proteins (HSP) can be cross-reactive among bacterial and human antigens. There is evidence that microbial HSP65 and human HSP60 are involved in periodontal disease. The aim of this study is to investigate immune responses to the human HSP60 and microbial HSP65 in patients with CP and relate these to the level of inflammation and smoking status. We collected serum samples from 30 patients with chronic gingivitis (CG) and 30 patients with CP. In each group, eight subjects were current smokers. ELISA was used to determine the levels of serum anti-HSP and C-reactive protein (CRP) in each group. Peripheral blood mononuclear cells were also isolated and stimulated with HSPs. Significant lymphoproliferation was seen in CP when stimulated with human HSP60. CRP and serum anti-human HSP60 IgG were elevated in CP compared to the CG, but not serum anti-microbial HSP 65 IgG. In view of the potential confounding effects of smoking in CP, a group of current smokers (n = 16) was also recruited to investigate whether smoking affects HSP immune responses. There was no significant difference in HSP-induced lymphoproliferation between smokers and non-smokers in either the CG or CP. There was a significant correlation between CRP and lymphoproliferative responses to Human HSP60 irrespective of smoking status. This study shows that serum anti-human HSP60 IgG and serum CRP are raised in untreated CP. In CP, serum CRP levels correlated significantly with human HSP60-induced lymphoproliferation, but not with anti-HSP antibody levels.

熊果酸干预人牙周膜干细胞成骨分化的效应

背景:熊果酸可促进骨髓间充质干细胞向成骨细胞定向分化,但其对人牙周膜干细胞是否具有促成骨作用目前相关报道少见。目的:探讨熊果酸对人牙周膜干细胞增殖和成骨分化能力的影响。方法:分离、培养人牙周膜干细胞,取第3代细胞,分别采用含不同浓度(0,1,2,4,6,8μmol/L)熊果酸的普通培养基干预,干预1,3,5,7 d后,采用CCK-8法检测细胞增殖,筛选适宜干预浓度。取第3代人牙周膜干细胞,分别用含0,1,2,4μmol/L熊果酸的成骨诱导液干预,干预7 d后,采用qRT-PCR法检测碱性磷酸酶、Runx2、骨钙素m RNA的表达,干预14 d后,茜素红染色观察矿化结节形成。取第3代人牙周膜干细胞,对照组加入成骨诱导液,熊果酸组、拮抗剂组分别加入含熊果酸(2μmol/L)、骨形态发生蛋白信号通路拮抗剂Noggin的成骨诱导液,熊果酸+拮抗剂组加入含熊果酸(2μmol/L)、骨形态发生蛋白信号通路抑制剂Noggin的成骨诱导液,培养7 d后,采用qRT-PCR和Western blot检测骨形态发生蛋白2、Smad1、骨桥蛋白、Runx2的m RNA及蛋白表达。结果与结论:(1)1,2,4μmol/L熊果酸可促进人牙周膜干细胞的增殖,6,8μmol/L熊果酸可抑制人牙周膜干细胞的增殖,后续实验选择1,2,4μmol/L熊果酸进行干预;(2)与0μmol/L相比,1,2,4μmol/L熊果酸可促进碱性磷酸酶、Runx2、骨钙素m RNA的表达以及矿化结节的形成(P<0.05),其中以2μmol/L熊果酸效果最显著;(3)与对照组比较,熊果酸组骨形态发生蛋白2、Smad1、骨桥蛋白、Runx2的mRNA及蛋白表达均升高(P<0.05),拮抗剂组上述指标的mRNA及蛋白表达均降低(P<0.05);与熊果酸组比较,熊果酸+拮抗剂组上述指标的mRNA及蛋白表达均降低(P<0.05);(4)结果表明,熊果酸可通过激活骨形态发生蛋白信号通路促进人牙周膜干细胞的成骨分化。

Identification of the Disrupted Pathways Associated with Periodontitis Based on Human Pathway Network

Objective: The objective of this work is to search for a novel method to explore the disrupted pathways associated with periodontitis(PD) based on the network level.Methods: Firstly, the differential expression genes(DEGs) between PD patients and cognitively normal subjects were inferred based on LIMMA package. Then, the proteinprotein interactions(PPI) in each pathway were explored by Empirical Bayesian(EB) coexpression program. Specifically, we determined the 100 th weight value as the threshold value of the disrupted pathways of PPI by constructing the randomly model and confirmed the weight value of each pathway. Meanwhile, we dissected the disrupted pathways under the weight value > the threshold value. Pathways enrichment analyses of DEGs were carried out based on Expression Analysis Systematic Explored(EASE) test. Finally, the better method was selected based on the more rich and significant obtained pathways by comparing the two methods. Results: After the calculation of LIMMA package, we estimated 524 DEGs in all. Then we determined 0.115222 as the threshold value of the disrupted pathways of PPI. When the weight value>0.115222, there were 258 disrupted pathways of PPI enriched in. Additionally, we observed those 524 DEGs that were enriched in 4 pathways under EASE=0.1.Conclusion: We proposed a novel network method inferring the disrupted pathway for PD. The disrupted pathways might be underlying biomarkers for treatment associated with PD.

Cytokines Elicited by HSP60 in Periodontitis with and without Coronary Heart Disease

The human 60 kDa and microbial 65 kDa heat shock proteins (HSP) have been implicated in the pathogenesis of chronic periodontitis (CP) and coronary heart disease (CHD). We have studied 100 subjects: Group (a) consisted of patients with gingivitis (n = 25), group (b) were patients with CP (n = 25), group (c) patients with CHD and gingivitis (n = 25) and group (d) patients with CHD and CP (n = 25). PBMCs separated from peripheral blood were stimulated with medium, PMA/ionomycin, human HSP60, microbial HSP65, or no stimulus for 18 hours before intracellular IL-2, IFN-γ, TNF-α, IL-4, IL-5, or IL-17 were detected by flow cytometry. The mean fluorescence intensity (MFLI) for intracellular TNF-α was significantly increased when PBMC were stimulated with human HSP60 amongst the four groups (p = 0.001, ANOVA);pairwise comparisons revealed significant differences in MFLI between the gingivitis group and the CP (p = 0.017);between gingivitis and ging/CHD (p = 0.001) as well;but no significant difference between the CP and CP/CHD (p = 0.442). There was no significant difference in intracellular expression of IL-17, or any of the other cytokines tested;and the MFLI for HSP-stimulated were comparable to unstimulated cultures. When heat-labile human HSP60 was heated, intracellular cellular TNF-α expression was abrogated. In contrast, heat-stable LPS elicited TNF-α expression from monocytes in bulk cultures in all groups. These results suggest that the cytokine expression was dependent on human HSP60 and not LPS. Serum CRP was significantly associated with MFLI of intracellular TNF-α in CP patients (rs = 0.665, p = 0.026) and CP/CHD (rs = 0.699, p = 0.011). We conclude that human HSP60 elicits increased monocytic expression of TNF-α in patients with CP, CP/CHD or ging/CHD compared to patients with gingivitis. Since the marker of inflammation, namely CRP correlates with CP with or without CHD and not with mild chronic gingivitis or ging/CHD, this suggests that human HSP60-induced production of TNF-α is associated with CP and not CHD. There was no significant difference in intracellular expression of IL-17.

血清HMGB1、CCL20、HSP27水平与慢性牙周炎患者牙周病变程度的相关性分析

目的探讨血清高迁移率族蛋白1(HMGB1)、CC趋化因子配体20(CCL20)、热休克蛋白27(HSP27)水平与慢性牙周炎(CP)患者牙周病变程度的相关性。方法选取2021年9月至2023年8月在新乡医学院第一附属医院诊治的60例CP患者纳入观察组,根据1∶1原则,另选取同期牙周健康者60例纳入对照组。比较两组及不同牙周病变程度CP患者血清HMGB1、CCL20、HSP27水平,分析各指标水平与CP牙周病变程度的相关性及联合诊断价值,并分析不同血清水平患者发生CP的危险度。结果观察组血清HMGB1、CCL20、HSP27水平高于对照组(P<0.05);不同牙周病变程度CP患者血清HMGB1、CCL20、HSP27水平比较:轻度<中度<重度,且各指标水平与牙周病变程度均呈正相关(P<0.05);入院时HMGB1、CCL20、HSP27水平联合诊断CP的曲线下面积(AUC)为0.905,最佳诊断敏感度为91.67%,特异度为88.33%,约登指数0.800,且各指标高水平患者发生CP的危险度是低水平的1.105倍、1.034倍、1.105倍(P<0.05)。结论HMGB1、CCL20、HSP27在CP患者血清中呈异常高表达,各指标水平与牙周病变程度均呈正相关,且联合检测对CP具有较高诊断价值,可作为临床诊断CP、评估牙周病变程度的有效指标。

miR-149-3p靶向调节Akt1介导牙周膜干细胞成骨分化的作用机制研究

目的探讨miR-149-3p靶向调节蛋白激酶B(protein kinase B,Akt1)介导牙周膜干细胞(periodontal ligament stem cells,PDLSCs)成骨分化的作用及机制。方法选取2022-01月在作者医院口腔科就诊的18~25岁患者因正畸而拔除的前磨牙或第三磨牙,分离牙周膜组织,提取人PDLSCs。免疫组织化学染色法检测角蛋白(pan-cytokeratin)和波形蛋白(vimentin)鉴定人PDLSCs。将人PDLSCs分为对照组、空载组、miR-149-3p inhibitor组和miR-149-3p mimic组。对照组人PDLSCs不进行处理,空载组、miR-149-3p inhibitor组和miR-149-3p mimic组按Lipofectamine 3000说明书方法分别将空载质粒和miR-149-3p inhibitor、miR-149-3p mimic转染到人PDLSCs。实时荧光逆转录聚合酶链反应(real-time reverse transcription polymerase chain reaction,RT-PCR)检测细胞内miR-149-3p、碱性磷酸酶(alkaline phosphatase,ALP)、Runt相关转录因子2(runt-related transcription factor 2,Runx2)、Akt1 mRNA表达;Western blot检测细胞内ALP、Runx2、Akt1蛋白表达。采用Fluo-3 AM探针检测细胞内钙离子。结果免疫组织化学结果显示,人PDLSCs二氨基联苯胺(diaminobenzidine,DAB)染色vimentin呈阳性,pan-cytokeratin呈阴性,提示PDLSCs提取成功。与对照组和空载组相比,miR-149-3p inhibitor组miR-149-3p表达显著降低,ALP、Runx2、Akt1 mRNA和蛋白表达、细胞内钙离子荧光强度均显著升高(P均<0.05);miR-149-3p mimic组miR-149-3p表达显著升高,ALP、Runx2、Akt1 mRNA和蛋白表达、细胞内钙离子荧光强度均显著降低(P均<0.05)。与miR-149-3p inhibitor组相比,miR-149-3p mimic组miR-149-3p表达显著升高,ALP、Runx2、Akt1 mRNA和蛋白表达、细胞内钙离子荧光强度均显著降低(P均<0.05)。对照组与空载组各指标比较差异均无统计学意义(P>0.05)。结论过表达miR-149-3p可靶向抑制Akt1蛋白的表达,从而抑制成骨标志物ALP和Runx2表达,降低人PDLSCs内钙离子浓度,不利于人PDLSCs成骨分化。

线粒体解偶联蛋白2在大鼠实验性牙周炎相关肾损伤中的作用研究

目的探索线粒体解偶联蛋白2(UCP2)在结扎诱导的实验性牙周炎相关肾损伤中的变化,研究UCP2对牙周炎诱导肾损伤的影响。方法选取12只Wistar雄性大鼠随机分为2组:对照组和牙周炎组。使用0.2 mm正畸结扎丝结扎在大鼠上颌第一磨牙的牙颈部,建立牙周炎模型。8周后观察2组大鼠口内情况,检测牙周临床指标牙龈出血指数(BI)、牙周探诊深度(PD)、牙齿松动度(TM)。收集大鼠上颌骨并扫描Micro CT,观察牙槽骨吸收情况,记录组织矿物质密度(TMD)、骨矿物质密度(BMD)、骨体积分数(BV/TV)、骨小梁厚度(Tb.Th)、骨小梁骨分离度(Tb.Sp)等参数,测量上颌第一磨牙釉牙骨质界到牙槽嵴顶的距离(CEJ-ABC)。冻存大鼠肾组织以检测氧化应激指标丙二醛(MDA)、谷胱甘肽(GSH)、超氧化物歧化酶(SOD),并进行实时定量聚合酶链反应(qRT-PCR)观察UCP2、核因子红系2相关因子2(Nrf2)抗体、过氧化物酶体增殖物激活受体γ辅激活因子-1α(PGC-1α)基因表达情况。使用大鼠牙龈组织进行免疫组织化学染色,观察牙龈组织UCP2表达情况。使用大鼠固定的肾组织进行苏木精-伊红(HE)、过碘酸雪夫(PAS)、MitoSOX Red、JC-1、免疫组织化学染色,观察大鼠肾组织病理学表现、活性氧(ROS)水平、线粒体膜电位水平及UCP2、Nrf2、PGC-1α蛋白表达情况。收集大鼠血清检测肾脏功能指标血尿素氮(BUN)、肌酐(Cre)、白蛋白(Alb)的表达。结果相较于对照组,牙周炎组大鼠第一磨牙周围的牙龈组织发红肿胀,质地松软,临床检查探诊出血且PD增加,牙齿松动,牙槽骨吸收,TMD、BMD、BV/TV、Tb.Th指数降低,Tb.Sp指数及CEJ-ABC增加,牙龈UCP2蛋白表达升高。相较于对照组,牙周炎组大鼠肾组织内MDA、ROS水平上升,MMP、GSH和SOD水平下降,UCP2基因及蛋白表达升高,Nrf2、PGC-1α基因及蛋白表达下降。肾脏功能指标BUN、Cre、Alb两组差异无统计学意义。结论UCP2可通过氧化应激在牙周炎诱导的肾损伤中发挥作用。

血清CCL21、CYTL-1水平与慢性牙周炎患者牙龈卟啉单胞菌感染及牙周临床指标的相关性

目的探讨血清趋化因子21(CCL21)、细胞因子样蛋白1(CYTL-1水平)与慢性牙周炎(CP)患者牙龈卟啉单胞菌(PG)感染及牙周临床指标的相关性。方法选取2019年6月至2023年5月在本院就诊的303例CP患者为实验组研究对象,并选取同期206例非CP患者作为对照组。根据CP患者病情严重程度分为轻度CP组(183例)、中度CP组(86例)、重度CP组(34例),分析患者一般资料及牙周指标的差异。检测血清中CCL21和CYTL-1表达水平。分析血清CCL21和CYTL-1表达水平与PG感染和牙周临床指标的相关性;采用ROC曲线分析CCL21和CYTL-1对CP的诊断价值。结果实验组PG的阳性率(68.32%)远高于对照组(17.96%)(P<0.05)。实验组中血清CCL21表达水平(270.82±33.77pg/mL)显著高于对照组(237.56±40.07pg/mL)(P<0.05),血清CYTL-1表达水平(174.41±29.85ng/mL)显著低于对照组(206.44±38.23ng/mL)(P<0.05)。随着CP患者病情的不断加重,PG的阳性率、血清CCL21表达水平和牙周指标呈现不同程度的上升趋势;而血清CYTL-1水平随着病情严重程度呈下降趋势(P<0.05)。CCL21表达水平与PG阳性感染和牙周指标均呈正相关(r=0.566、0.486、0.444、0.417、0.528,均P<0.05);CYTL-1表达水平与PG阳性感染和牙周指标均呈负相关(r=-0.584、-0.451、-0.433、-0.407、-0.456,均P<0.05);CCL21和CYTL-1两项者联合诊断CP结果优于任何一项单独分析(Z两项联合-CCL21=4.142,Z两项联合-CYTL-1=3.824;P<0.05)。结果CP患者血清中CCL21表达上调,CYTL-1表达下调与PG感染和牙周临床指标密切相关,且二者联合对CP有一定的诊断价值。

生物钟蛋白Bmal1对实验性牙周炎相关肾损伤的影响

目的通过建立大鼠牙周炎模型,探讨生物钟蛋白Bmal1对慢性牙周炎相关肾损伤的影响。方法将12只雄性Wistar大鼠随机分为对照组和牙周炎组,每组6只。采用正畸结扎丝对牙周炎组大鼠双侧上颌第一磨牙进行结扎处理,对照组大鼠不进行任何干预措施。8周后,检测2组大鼠的牙周临床指标,包括牙周探诊深度、牙龈出血指数和牙齿松动度。采用Micro-CT对大鼠上颌骨进行扫描和三维图像重建,评估牙槽骨吸收情况。采用苏木精-伊红(HE)和过碘酸雪夫(PAS)染色对牙周组织和肾组织进行病理学观察。采用生化试剂盒检测肾脏功能指标肌酐、白蛋白、血尿素氮的水平,以及氧化应激指标超氧化物歧化酶、谷胱甘肽和丙二醛的水平。MitoSOX red染色检测肾组织内活性氧(ROS)含量。实时荧光定量聚合酶链反应(RT-qPCR)和免疫组织化学染色检测大鼠肾组织中Bmal1、核因子-E2相关因子2(Nrf2)和血红素加氧酶1(HO-1)的基因及蛋白表达水平。结果与对照组相比,牙周组织Micro-CT及HE染色结果显示,牙周炎组上颌第一磨牙区出现明显的骨吸收和附着丧失;肾组织HE及PAS染色结果表明,牙周炎组大鼠肾组织有显著的组织病理损伤;肾功能和氧化应激指标结果显示,牙周炎组的氧化应激水平出现异常而肾功能指标无明显异常;MitoSOX red结果显示,牙周炎组肾组织内ROS含量升高;RT-qPCR和免疫组织化学结果显示,牙周炎组肾组织内Bmal1、Nrf2和HO-1表达水平降低。结论生物钟蛋白Bmal1在牙周炎大鼠肾脏的氧化损伤过程中发挥重要作用。

GSK3β/Fis1信号通路在甲基乙二醛诱导成骨细胞凋亡中的作用及机制

目的探讨糖原合成酶激酶3β(glycogen synthase kinase 3β,GSK3β)/线粒体分裂蛋白1(fission protein 1,Fis1)信号通路在甲基乙二醛(methylglyoxal,MG)诱导成骨细胞凋亡中的作用及机制。方法采用LiCl作为GSK3β抑制剂,将细胞随机分为4组,即对照组、MG组、LiCl组和LiCl+MG组。采用MTT法检测细胞增殖活性,Tunel染色法分析细胞凋亡情况,Western blot法检测GSK3β、Fis1蛋白表达水平,MitoTracker Deep Red染色法分析线粒体形态。结果MTT法检测结果表明,MG抑制了成骨细胞增殖活性。Tunel染色法检测结果显示,MG诱导成骨细胞凋亡。Western blot法检测结果表明,MG处理后GSK3β蛋白磷酸化水平降低,Fis1蛋白表达水平增加。MitoTracker Deep Red染色法分析结果显示,MG处理后线粒体呈碎片化。在加入GSK3β抑制剂LiCl干预后,与MG组比较,其显著恢复了MG抑制的细胞增殖活性、减少细胞凋亡,同时GSK3β蛋白磷酸化水平升高,Fis1蛋白表达水平降低,并且恢复了线粒体形态。结论MG可能通过调控GSK3β/Fis1信号通路促进线粒体分裂增加,诱导成骨细胞凋亡。

牙龈卟啉单胞菌促进阿尔茨海默病的机制研究进展

阿尔茨海默病(Alzheimer’s disease,AD)是最常见的神经退行性疾病之一。牙龈卟啉单胞菌(Porphyromonas gingivalis,P.gingivalis)感染与AD密切相关。本文综述了P.gingivalis及其毒力因子在AD发生发展过程中的多重作用及其机制,旨在深入阐明两者之间的内在联系。P.gingivalis可通过多种途径与AD发生发展相关联。首先,P.gingivalis可以增加神经炎症、促进淀粉样蛋白和Tau蛋白沉积、破坏血脑屏障等途径参与AD病理进程。其次,P.gingivalis分泌的牙龈蛋白酶能增加血脑屏障通透性并进入脑内诱导病理损伤是其促进AD的重要机制。临床样本检测也支持P.gingivalis或其效应分子促进AD病理进展。因此,P.gingivalis可能是AD的一个环境易感因素或可调控的风险因素。目前P.gingivalis在AD中的确切作用机制和P.gingivalis与其他可能影响AD的因素之间的关联研究不明确。本文深入分析P.gingivalis促进AD的分子机制,为研制P.gingivalis相关的AD新型防治策略提供参考。

Effects of Shuanghuangbu on the total protein content and ultrastructure in cultured human periodontal ligament cells

Background Successful periodontal regeneration depends on the migration, proliferation and differentiation of periodontal ligament cells in periodontal defects. The total protein content and the ultrastructure demonstrate the metabolizability and activity of periodontal ligament cells. This study was conducted to observe the effects of Shuanghuangbu, a mixture of medicin al herbs, on the total protein content and the ultrastructure of human periodontal ligament cells. Methods Periodontal ligament cells were grown to confluence and then cultured in Dulbecco’s modified eagle medium (DMEM) supplemented with Shuanghuangbu over the concentration range of 0 to 1000 μg/ml. The total protein content in cultured cells was determined by using Coommasie brilliant blue technique. Periodontal ligament cells were incubated in 0 and 100 μg/ml Shuanghuangbu decoction for 5 days, then observed through transmission electron microscope.Results The total protein content of human periodontal ligament cells increased in each experiment group added 10-1000 μg/ml Shuanghuangbu respectively, and the effect of 100 μg/ml was excellent. Under the transmission electron microscope, there were more rough endoplasmic reticulums and mitochodrias in the experiment group than those in the control group. Conclusion Shuanghuangbu stimulates the protein synthesis of human periodontal ligament cells and improves human periodontal ligament cells’ metabolizability and activity.

敲除巨噬细胞Zfp260通过抑制M1型极化减轻小鼠牙周炎症

目的:研究锌指蛋白260(zinc finger protein 260,Zfp260/ZNF260)对巨噬细胞极化和牙周炎牙槽骨吸收的影响。方法:实时定量聚合酶链反应(real-time quantitative polymerase chain reaction,RT-qPCR)检测人/野生型小鼠炎症牙周组织中ZNF260/Zfp260的表达。RT-qPCR检测RAW264.7细胞在炎症和非炎症环境中Zfp260的表达。繁育巨噬细胞内特异性敲除Zfp260小鼠,分别构建flox/flox对照鼠(Zfp260^(f/f);Lyz2-cre^(-))和条件性敲除(conditional knockout,cKO)鼠(Zfp260^(f/f);Lyz2-cre^(+))牙周炎模型,micro-CT、苏木精-伊红(hematoxylin and eosin,HE)染色观察牙槽骨形态变化。RT-qPCR、蛋白质印迹法观察应用特异性小干扰RNA(small interfering RNA,siRNA)沉默Zfp260表达对RAW264.7极化的影响。RT-qPCR、免疫荧光染色观察牙周组织中M1、M2型极化标志分子的表达。结果:人/野生型小鼠炎症牙周组织中ZNF260/Zfp260的表达明显高于健康组。炎症环境下RAW264.7细胞中Zfp260的表达明显上调。cKO小鼠的牙周炎侧骨吸收小于flox/flox小鼠。沉默Zfp260表达可抑制RAW264.7在炎症环境下的M1型极化,且cKO小鼠的炎症牙周组织中M1型极化标志分子的表达明显少于flox/flox小鼠。结论:干扰巨噬细胞Zfp260的表达可抑制M1型极化并减轻牙周炎导致的牙槽骨吸收。

莱菔子提取物基于PI3K/AKT信号通路改善糖尿病牙周炎大鼠炎症反应的作用研究

目的探究莱菔子提取物在糖尿病牙周炎大鼠模型中对牙周炎症的改善作用并分析其与PI3K/AKT信号通路之间的关联性。方法40只SD雄性大鼠随机等量分为5组:空白对照组(N组)、牙周炎模型组(P组)、牙周炎莱菔子治疗组(P+Q组)、糖尿病牙周炎模型组(DP组)、糖尿病牙周炎莱菔子治疗组(DP+Q组)。除N组外,其余4组大鼠均通过口腔正畸丝牙周结扎法与菌液涂布法联合建立牙周炎模型;DP组和DP+Q组辅以一次性腹腔注射链脲佐菌素建立糖尿病牙周炎模型。建模成功后,P+Q组和DP+Q组通过灌胃给药的方式分别给予莱菔子提取物2.5g/(kg·d),N组、P组和DP组则给予等量生理盐水。连续给药8周,过程中观察大鼠一般状况并跟踪大鼠的空腹血糖变化。给药结束后处死取材,处死前记录大鼠牙龈指数、龈沟出血指数;记录牙槽骨吸收高度;利用酶联免疫吸附法检测血清中白细胞介素-6和肿瘤坏死因子-α水平;采用苏木精-伊红染色观察并比较大鼠牙周组织病理形态变化;运用Western blot法测定大鼠牙周组织中PI3K/AKT信号通路中相关蛋白的表达水平。结果P组和DP组白细胞介素-6和肿瘤坏死因子-α水平显著高于N组,DP组白细胞介素-6和肿瘤坏死因子-α水平显著高于P组(P<0.05)。P+Q组和DP+Q组白细胞介素-6和肿瘤坏死因子-α水平分别低于P组和DP组(P<0.05)。DP组PI3K、AKT表达量显著低于N组(P<0.05)。DP+Q组PI3K、AKT表达量显著高于DP组(P<0.05)。结论莱菔子提取物可基于PI3K/AKT信号通路改善糖尿病牙周炎大鼠炎症反应,保护牙周组织。

2型糖尿病合并牙周炎老年患者血清炎症及氧化应激水平与牙周参数的相关性

目的 探讨2型糖尿病(T2DM)合并牙周炎老年患者血清糖基化终末产物(AGE)、C反应蛋白(CRP)、丙二醛(MDA)水平与牙周参数的相关性。方法 选择2021年6月至2022年10月濮阳市人民医院口腔科T2DM合并牙周炎老年患者45例作为T2DM牙周炎组,并选择同期老年健康体检者45例作为对照组,牙周炎老年患者45例作为单纯牙周炎组。比较入选患者一般资料、牙周参数[探诊深度(PD)、龈沟出血指数(SBI)]、血清因子指标(AGE、CRP、MDA),采用Pearson分析血清AGE、CRP、MDA水平与牙周参数的相关性。结果 单纯牙周炎组、T2DM牙周炎组PD、SBI高于对照组,T2DM牙周炎组PD、SBI高于单纯牙周炎组(P <0.05)。单纯牙周炎组、T2DM牙周炎组血清AGE、CRP、MDA水平高于对照组,T2DM牙周炎组血清AGE、CRP、MDA水平高于单纯牙周炎组(P <0.05)。Pearson相关性显示,血清AGE、CRP与PD之间存在强相关性(r=0.611,P <0.001;r=0.646,P <0.001),血清MDA与PD之间存在中等程度相关(r=0.554,P <0.001);血清AGE与SBI之间存在中等程度相关(r=0.575,P<0.001),血清CRP、MDA与SBI之间存在强相关性(r=0.691,P<0.001;r=0.689,P <0.001)。结论 T2DM合并牙周炎老年患者血清AGE、CRP、MDA水平明显升高,且上述指标水平与牙周参数PD、SBI呈正相关关系。