简介：糖尿病已成为我国主要的公共卫生问题,糖尿病性视网膜病变（diabeticretinopathy,DR）是一种严重的致盲眼病,如不及时治疗将会造成不可逆的永久性损害。

简介：目的了解安阳县≥40岁自觉视力障碍的农民盲与低视力的患病率及致盲原因.方法安阳县各行政村中,≥40岁自觉视力障碍的农民为筛查对象.采用WHO盲与低视力标准和白内障诊断标准.由眼科医生作眼部检查.对所有视力＜0.3的患眼进行主要病因诊断,确诊所有白内障患者,并筛选出需手术治疗者.结果共检查853例,盲目患者23例,患病率2.70%,低视力患者99例,患病率4.27%,致盲的主要眼病依次为白内障、角膜病、青光眼、视网膜病等.共筛查出533例白内障,行白内障手术治疗301人次,脱残率98%,脱盲率99.34%.结论白内障仍是盲和低视力的首要病因,防盲治盲的重点仍是白内障复明手术.

简介：目的：对一个常染色体显性遗传的先天性脉络膜缺损家系进行ABCB6基因的突变筛查,明确致病基因。方法：近来有报道ABCB6基因突变可导致先天性脉络膜缺损,我们搜集了一个中国汉族先天性脉络膜缺损家系,采集家系成员及一百位正常对照人群的静脉血5mL,使用PCR产物直接测序对ABCB6基因进行突变筛查。结果：在该家系中我们发现了一个新突变（c.1380c〉a）,该突变在家系中与疾病表型共分离,并且在100名正常对照中均未发现该突变。结论：我们的研究结果扩大了ABCB6基因的突变谱,进一步确认了该基因在眼组织缺损发病中发挥了重要作用。

简介：目的评价带线羟基磷灰石义眼座(HA)无包裹植入的临床疗效.方法对29例眼球摘除术后患者,采用带线羟基磷灰石义眼座作为眼窝植入物,无包裹直接植入.Ⅰ期植入21例.Ⅱ期植入8例.结果分别随访5-18月,4眼术后出现球结膜裂开,2眼术后轻度上睑下垂,1眼术后五月义眼座中度暴露,均经相应治疗后恢复.其他病例手术效果良好,无植入物脱出及移位,义眼座活动度良好.结论带线羟基磷灰石义眼座直接植入术,具有操作简单、材料易得、并发症少等优点,具有良好的应用前景.

简介：目的：研究近视患者LASIK术后视疲劳的发生与融合范围的关系，及同视机融合功能训练改善LASIK术后视疲劳的疗效观察。方法：对60例120眼近视患者（．1．50--8．00D）施行LASIK手术，于术前戴全矫眼镜用同视机法测定融合范围，并进行视疲劳的问卷调查。术后将其随机平分为两组：A组进行同视机融合功能训练30d，B组不进行同视机融合功能训练，分别对其术后1wk；1mo行同视机法测定融合范围，并进行视疲劳的问卷调查及统计学分析。结果：A、B组术后融合范围均较术前减小。术后1wk时融合范围两组分别为18．58±8．91和13．45±8．87，二者差异有统计学意义（P〈0．05）。术后1mo时，两组融合范围分别为20．55±7．23和18．12±6．10，二者差异无统计学意义。术后1wk时A组视疲劳评分3．92±1．65，B组评分5．16±2．34，二者差异有统计学意义（P〈0．05）。术后1mo时两组评分分别是1．28±0．96和1．45±0．99分，二者差异无统计学意义。结论：近视眼LASIK术后双眼的融合功能下降是出现视疲劳的一个重要因素。术后早期进行同视机融合功能训练可以有效的改善视疲劳症状。

简介：AIM:Tocomparetheregularityandaccuracyoflaserinsitukeratomileusis(LASIK)flapscreatedbytheZiemerFEMTOLDV'Classic'(Ziemer'Classic')andZiemerFEMTOLDVCrystalLinefemtosecondlaser(ZiemerCrystalLine).METHODS:Fourier-domainopticalcoherencetomography(RTVueOCT)wasusedtomeasurethemorphologyof200LASIKflapsof100consecutivepatientscreatedwiththeZiemerClassic(100flaps)ortheZiemerCrystalLine(100flaps)atoneweekpostoperatively.Flapthicknesswasevaluatedat36specifiedmeasurementpointsoneachflap.Forallprocedureswithbothlasers,thenominalflapthicknesswas110μm.RESULTS:ThemeanflapthicknessoftheZiemerCrystalLinegroup(102.49±2.68μm)wasthinnerthanthatoftheZiemerClassicgroup(107.65±5.09μm)(P<0.01).Averagethicknessofallflapswasuniformwithin4μmatallmeasurementpoints.TheflapsintheZiemerCrystalLinegroupweremoreregularthanthoseintheZiemerClassicgroupwhenmeasuredfromthecentertotheperiphery.Themaximumdeviationfromthenominal110μmof36measurementswas8μmintheZiemerClassicgroup,whileintheZiemerCrystalLinegroupitwas9μm.Withinthe3600measurementsonthe100eyes,differencesgreaterthan20μmwereobserved0.14%intheZiemerClassicgroup,and0.04%intheZiemerCrystalLinegroup.CONCLUSION:TheflapscreatedwiththeZiemerFEMTOLDVCrystalLinefemtosecondlaseraremoreuniformandthinnerthanthosecreatedbytheZiemerFEMTOLDVClassicfemtosecondlaser.

简介：AIM:Toestablishanuntransfectedhumancornealstromal(HCS)celllineandcharacterizeitsbiocompatibilitytoacellularporcinecornealstroma(aPCS).·METHODS:PrimaryculturewasinitiatedwithapurepopulationofHCScellsinDMEM/F12media(pH7.2)containing20%fetalbovineserumandvariousnecessarygrowthfactors.Theestablishedcelllinewascharacterizedbygrowthproperty,chromosomeanalysis,tumorigenicityassay,expressionofmarkerproteinsandfunctionalproteins.Furthermore,thebiocompatibilityofHCScellswithaPCSwasexaminedthroughhistologicalandimmunocytochemistryanalysesandwithlight,electronmicroscopies.·RESULTS:HCScellsproliferatedtoconfluence2weekslaterinprimarycultureandhavebeensubculturedtopassage140sofar.AcontinuousuntransfectedHCScelllinewithapopulationdoublingtimeof41.44hoursatpassage80hasbeendetermined.Resultsofchromosomeanalysis,morphology,combinedwiththeresultsofexpressionofmarkerproteinandfunctionalproteinssuggestedthatthecellsretainedHCScellproperties.Furthermore,HCScellshavenotumorigenicity,andwithexcellentbiocompatibilitytoaPCS.·CONCLUSION:Anuntransfectedandnon-tumorigenicHCScelllinehasbeenestablished,andthecellsmaintainedpositiveexpressionofmarkerproteinsandfunctionalproteins.Thecellline,withexcellentbiocompatibilitytoaPCS,mightbeusedforinvitroreconstructionoftissue-engineeredHCS.

简介：AIM:Todemonstratethemorphologyandstructureofinvitroreconstructedtissue-engineeredhumancornealepithelium(TE-HCEP)withseedercellsfromanuntransfectedHCEPcellline.·METHODS:TheTE-HCEPswerereconstructedinvitrowithseedercellsfromanuntransfectedHCEPcellline,andscaffoldcarriersofdenudedamnioticmembrane(dAM)inair-liquidinterfaceculturefor3,5,7and9days,respectively.Thespecimenswereexaminedwithhematoxylin-eosin(HE)stainingofparaffin-section,immunocytochemicalstaining,scanningandtransmissionelectronmicroscopy.·RESULTS:DuringinvitroreconstructionofTE-HCEP,HCEPcellsformeda3-4,6-7and8-10layersofanHCEP-likestructureondAMsinair-liquidinterfaceculturefor3,5and7days,respectively.Butthecellsdeceasedto5-6layersandthestructureofstraifiedepitheliumbecamelooseatday9.Andthecellsmaintainedpositiveexpressionofmarkerproteins(keratin3andkeratin12),cell-junctionproteins(zonulaoccludens-1,E-cadherin,connexin43andintegrinβ1)andmembranetransportproteinofNa+-K+ATPase.TheHCEPcellsinTE-HCEPwererichinmicrovillionapicalsurfaceandestablishednumerouscell-cellandcell-dAMjunctionsatday5.·CONCLUSION:ThemorphologyandstructureofthereconstructedTE-HCEPweresimilartothoseofHCEPinvivo.TheHCEPcellsinthereconstructedTE-HCEPmaintainedthepropertiesofHCEPcells,includingabilitiesofformingintercellularandcell-extracellularmatrixjunctionsandabilitiesofperformingmembranetransportation.TheuntransfectedHCEPcellsanddAMscouldpromisinglybeusedinreconstructionHCEPequivalentforclinicalcornealepitheliumtransplantation.