扬子鳄β防御素基因的血液表达谱及饲养密度对防御素基因表达的影响

为研究扬子鳄血液中β防御素基因家族的表达水平和饲养密度对群体防御素基因表达的影响,利用反转录荧光定量聚合酶链式反应(reverse transcription quantitative polymerase chain reaction,RT-qPCR)技术检测41头扬子鳄七龄鳄血液中β防御素基因的表达情况,并分析不同性别和不同饲养密度群体间防御素基因相对表达量的差异。结果表明:在扬子鳄群体血液中,表达的防御素基因有AsBD5和AsBD8,并且这2个基因的表达量之间存在显著的正相关性。AsBD5和AsBD8在雌性和雄性扬子鳄间的表达水平没有显著性差异;但是在不同饲养密度下,2个扬子鳄群体间的表达水平存在显著差异,其中饲养密度较高的扬子鳄群体,整体的防御素表达水平更高,表明饲养密度对扬子鳄圈养种群的免疫状态有一定的影响。

β防御素1基因单核苷酸多态性与呼吸机相关性肺炎易感性及预后的相关性研究

目的探讨β防御素1(HBD1)基因第一外显子5'非编码区(-52A/G、-44C/G、-20A/G)的单核苷酸多态性与呼吸机相关性肺炎(VAP)易感性和转归的相关性。方法 130例术后并发VAP的患者,设为VAP组;80例术后未并发VAP的患者,设为对照组;基因组DNA提取后,采用聚合酶链反应(PCR)扩增DNA片段及DNA直接测序的方法,测定HBD1基因第一外显子5'非编码区(-52A/G、-44C/G、-20A/G)单核苷酸多态性的基因型。结果 5'非编码区-52A/G、-44C/G、-20A/G位点均检测到3种基因型,VAP组患者HBD1基因-44C/G位点C和G等位基因的携带频率分别为81.5%和18.5%,而在对照组分别为90.6%和9.4%,两者比较差异有统计学意义(P<0.05),VAP组中,死亡组-44C/G位点C和G等位基因的携带频率,分别为60.0%、40.0%,而在存活组分别为84.1%、15.9%,两者比较差异有统计学意义(P<0.05),其余两个位点的基因型频率和等位基因频率,在VAP组、对照组及死亡组、存活组之间差异无统计学意义。结论 HBD1基因-44C/G位点单核苷酸多态性与VAP的易感性和转归相关,G等位基因为VAP易感和死亡的预警指标。

人β防御素3基因转染及金纳米颗粒处理后的牙周膜细胞对大鼠牙周炎形成影响研究

目的探讨人β防御素3基因转染大鼠牙周膜细胞,并经金纳米颗粒处理后,局部注射对SD大鼠慢性牙周炎形成的影响。方法丝线结扎法构建SD大鼠慢性牙周炎模型,酶消化法提取大鼠牙周膜细胞并鉴定,用携带人β防御素3基因的腺病毒转染细胞并经金纳米颗粒处理,在慢性牙周炎构建同期局部注射细胞悬液到腭侧牙龈,对照组分别注射生理盐水和空载体腺病毒转染后的细胞悬液。2周后处死大鼠取材。通过Micro-CT和免疫组化染色观察大鼠牙周炎形成情况。结果单纯结扎组第二磨牙周围牙槽骨明显吸收,牙龈上皮钉突向内增生,棘层增厚,炎细胞浸润,胶原纤维变性、局部断裂。局部注射经转染和金纳米颗粒处理的牙周膜细胞后,结扎区域牙槽骨吸收水平降低,骨密度和骨体积分数增加;牙龈上皮炎症细胞浸润和上皮钉突增生减少,胶原纤维断裂和排列紊乱等病理变化得到改善。结论人β防御素3基因转染及金纳米颗粒处理后的大鼠牙周膜细胞局部注射后,可减轻SD大鼠的牙周组织炎症,降低牙周组织破坏,从而在牙周炎的形成过程中起到保护作用。

EXPRESSION OF HUMAN BETA-DEFENSIN 3 IN COS-7 CELL

To establish a cell line for stable expression of human beta-defensin 3 (hBD3). Methods Full length cDNA of hBD3 was isolated from previously constructed pGEM-hBD3 and then inserted into pcDNA3. The recombinant vector identified carrying hBD3 with right direction was introduced into COS-7 cells by Lipofe-ctamine. Cell clones survived in G418-rich medium and with stable expression of hBD3 in both mRNA and protein levels were identified by RT-PCR and Western blot respectively. Genomic integration of the hBD3 gene with the COS-7 cells was confirmed by Southern dot blot and primary analysis. The antimicrobial activity of the secreted hBD3 was also evaluated. Results COS-7 cells transfected with pcDNA3-hBD3 expressed hBD3 stably in mRNA and protein level. Southern dot blot analysis showed successful integration of the hBD3 gene into the genome of COS-7 cell and the hBD-3 protein secreted into the culture medium showed antimicrobial activity. Conclusion We successfully established a hBD3-expressing cell line.