华南农业大学学报
華南農業大學學報
화남농업대학학보
JOURNAL OF SOUTH CHINA AGRICULTURAL UNIVERSITY
2015年
2期
79-84
,共6页
施琼%胡峰%黄烈健%陈应彪
施瓊%鬍峰%黃烈健%陳應彪
시경%호봉%황렬건%진응표
马大杂种相思%组织培养%有效增殖倍数
馬大雜種相思%組織培養%有效增殖倍數
마대잡충상사%조직배양%유효증식배수
Acacia mangium ×A.auriculiformis%tissue culture%proliferation index
目的提高马大杂种相思Acacia mangium ×A.auriculiformis良种的快速繁殖效率与推广种植力度.方法以马大杂种相思新生枝条带腋芽茎段为外植体,研究马大杂种相思组培快繁体系.结果和结论用质量分数为0.1%的升汞和体积分数为75%的乙醇分别处理当年新生枝条第3~5个腋芽茎段15 min和30 s,然后接种至MS培养基进行初代培养,芽诱导率为95.68%;最佳增殖培养基为改良MS+6-BA 1.5 mg· L-1+NAA 0.1 mg· L-1+蔗糖30~40 g· L-1,35 d的有效增殖倍数为3.97;将增殖芽接入含IBA 600 mg· L-1的MS固体培养基上预培养4~8 h后转接至无激素1/2 MS培养基上,15 d即可全部生根;或将增殖芽直接接入1/2 MS+IBA 1.0 mg · L-1+NAA 0.5 mg· L-1+蔗糖30 g· L-1生根培养基上,第15天时生根率为99.43%.将生根苗移栽至以黄心土为基质的营养袋内,存活率为94.67%.
目的提高馬大雜種相思Acacia mangium ×A.auriculiformis良種的快速繁殖效率與推廣種植力度.方法以馬大雜種相思新生枝條帶腋芽莖段為外植體,研究馬大雜種相思組培快繁體繫.結果和結論用質量分數為0.1%的升汞和體積分數為75%的乙醇分彆處理噹年新生枝條第3~5箇腋芽莖段15 min和30 s,然後接種至MS培養基進行初代培養,芽誘導率為95.68%;最佳增殖培養基為改良MS+6-BA 1.5 mg· L-1+NAA 0.1 mg· L-1+蔗糖30~40 g· L-1,35 d的有效增殖倍數為3.97;將增殖芽接入含IBA 600 mg· L-1的MS固體培養基上預培養4~8 h後轉接至無激素1/2 MS培養基上,15 d即可全部生根;或將增殖芽直接接入1/2 MS+IBA 1.0 mg · L-1+NAA 0.5 mg· L-1+蔗糖30 g· L-1生根培養基上,第15天時生根率為99.43%.將生根苗移栽至以黃心土為基質的營養袋內,存活率為94.67%.
목적제고마대잡충상사Acacia mangium ×A.auriculiformis량충적쾌속번식효솔여추엄충식력도.방법이마대잡충상사신생지조대액아경단위외식체,연구마대잡충상사조배쾌번체계.결과화결론용질량분수위0.1%적승홍화체적분수위75%적을순분별처리당년신생지조제3~5개액아경단15 min화30 s,연후접충지MS배양기진행초대배양,아유도솔위95.68%;최가증식배양기위개량MS+6-BA 1.5 mg· L-1+NAA 0.1 mg· L-1+자당30~40 g· L-1,35 d적유효증식배수위3.97;장증식아접입함IBA 600 mg· L-1적MS고체배양기상예배양4~8 h후전접지무격소1/2 MS배양기상,15 d즉가전부생근;혹장증식아직접접입1/2 MS+IBA 1.0 mg · L-1+NAA 0.5 mg· L-1+자당30 g· L-1생근배양기상,제15천시생근솔위99.43%.장생근묘이재지이황심토위기질적영양대내,존활솔위94.67%.
Objective]To improve the propagation efficiency and extend the planting of Acacia mangium × A.auriculiformis.[Method]This study was carried out to explore the techniques of in vitro propagation of A.mangium ×A.auriculiformis using stem segments with buds collected from 16-year plants as the ex-plant .[Result and conclusion]Current season stem segments carrying 3-5 axillary buds were sterilized with w=0.1%mercuric chloride and φ=75%alcoho1 for 15 min and 30 s respectively before they were inoculated onto MS medium .Buds could be induced successfully on MS with a shooting rate of 95.68%. The bud proliferation index was 3.97 after being transferred onto MS +6-BA 1.5 mg· L-1 +NAA 0.1 mg· L-1 +sucrose 30-40 g· L-1 for 35 d.The buds all rooted on the 15th day from inoculation onto 1/2 MS medium after pre-cultured on MS supplemented with IBA 600 mg· L-1 for 4-8 h.Inoculating the proliferated buds onto 1/2 MS+IBA 1.0 mg· L-1 +NAA 0.5 mg· L-1 +sucrose 30 g· L-1 also generated a high rooting rate of 99.43%.The survival rate reach 94.67% after the rooted plantlet are transplanted to the yellow soil medium .
