[摘要] Previousstudieshaveshownthatembryoniclensepithelialcellsofseveralspeciesofvertebrateselongateinculture,asdolenscellswhentheyformfibersinvivo.Otherstudieshaveshownthatmaturelensepithelialcellsdivideratherthanelongateinculture.Todetermineifandwhenduringdevelopmentlensepithelialcellschangeintheirabilitytoelongateinculture,thecentralregionsofembryonicchicklensepitheliawereexplantedatprogressivelylaterstagesofdevelopmentandexaminedhistologicallyafter3daysofcultivation.Cellsfrom6-,9-,12-,and15-day-oldembryoselongatedinculture.Theamountsofthymidine-CH3î—¸3Handofadenosine-2-3HincorporatedintoDNA,thepercentageofnucleilabeledwiththymidine-CH3î—¸3Handthepercentageofcellswithmitoticfiguresdecreasedaftercultureofexplantsfrom6-day-oldembryos.Bycontrast,epithelialcellstakenfrom19-day-oldembryosdidnotelongateinculture,andshowedanincreaseaftercultureintheamountsofthymidine-CH3î—¸3Handofadenosine-2-3HincorporatedintoDNA,inthepercentageofnucleilabeledwiththymidine-CH3î—¸3Handinthepercentageofcellswithmitoticfigures.Thus,theabilityoflensepithelialcellstoelongateincultureislostbetweenday15andday19ofdevelopmentofthechickembryo.