虎舌红组织培养技术体系研究
|
摘要
本研究力求探索虎舌红(Ardisia Mamillata Hance)组织培养快速繁殖的有效途径。以虎舌红的叶片、叶柄、茎尖、带芽茎段为外植体,着重研究其培养的最佳培养基配方及培养程序,建立虎舌红快繁技术体系。结果表明:
1)虎舌红组培条件为温度25±2℃,每天光照14h,光强1500~2000lux左右。
2)虎舌红组织培养快速繁殖的外植体以嫩叶(具有主叶脉)或顶芽或侧芽为好,最佳取材时间为3月中旬。
3)外植体消毒灭菌的有效方法是:先用肥皂水浸洗后,再用自来水冲洗1~2小时,冲洗干净后,晾干,切取其茎段、芽、嫩叶和叶柄分别放入装有75%酒精的烧杯中浸30s后取出,放入0.1%的升汞中消毒8min,在无菌条件下取出,用无菌水冲洗4~6次,为了冲洗掉残留的(Hg~(2+)),每次无菌水冲洗时间不少于2分钟,并不停地振荡,以便无菌水与材料充分接触。接种时,用干净滤纸吸干外植体表面水分,可以明显减少污染率和褐变率。
4)初代培养:芽萌发的最佳培养基为:2/3MS+BA2mg/L+IBA0.2mg/L+蔗糖3%,萌发率为91.0%;愈伤组织诱导的最佳培养基为MS+BA1.0mg/L+2,4-D1.0mg/L+蔗糖3%或MS+BA0.2mg/L+NAA0.2mg/L+2,4-D0.5mg/L+蔗糖3%,诱导效果较好,愈伤组织诱导率分别为75.19%,67.72%。
5)继代培养:芽苗增殖最佳培养基为MS+BA1.5mg/L+NAA0.1mg/L+蔗糖3%,增殖系数可达6.6,且芽苗生长良好。
6)生根培养:生根培养基以1/2MS+IBA0.5mg/L+NAA0.5mg/L+蔗糖2%为好,生根率达93.6%。在此培养基上添加不同浓度的活性炭,以0.2%AC效果更好。
7)炼苗:在基质选择上,珍珠岩与蛭石1:1混和炼苗成活率最高(64.4%),腐殖质土次之(53.3%),而纯砂最差(35%)。
8)试验结果按最佳处理计算,繁殖系数以30~40天左右为一个增殖周期,增殖系数为6~7,年理论增殖倍数可达2.8×10~8,能够在短期内达到大量增殖的目的。
Studies were carried out to find out the best composition of medium and propagation procedure by using the explants of terminal buds, axillary's buds, leaves of Ardisia Mamillata Hance. The results were as follows:
1)Culture conditions: temperature 25 2 , 14 hours illumination every day, and about 1500 Lux illumination intensity.
2)The optimal explants were young leaves (with partial main vein), shoot tips of terminal buds or lateral buds in middle March.
3)Effective surface sterilization of the primary explants was to soak them in 0.1% mercuric chloride for 8 minutes after washed in tap water for 1 ~2 hours and sterilized in 75% alcohol for 30 secends. Bloting the cultured material could prevent browning effectively when inoculating it on callus-inducing culture medium.
4)Primary cultivation: The best medium for bud's sprouting in initiation culture was 2/3MS+BA2mg/L+IBA0.2 mg/L in which sprouting rate could reach 91%. The best Callus-inducing culture medium was MS+BAlmg/L+2,4-D1.0mg/L or MS+ BA0.2mg/L +NAA0.2 mg/L +2, 4-D 0.5mg/L. Callus-inducing rate were 75.19% and 67.72% respectively.
5)The best subculture medium was MS+BA1.5mg/L+NAA0.1 mg/L+sucrose3%.
Where the multiplication rate was 6.6 or 2.8 108 per year.
6)The best rooting medium was l/2MS+IBA0.5mg/L+NAA0.5 mg/L +sugar2% +0.2%AC. Where the rooting rate could reach 93.6%.
7)Training seedling: The survial rate could reach 64.4% when the hardened rooted test tube plants were transplanted into the medium with 1/2 vermiculite and 1/2 ruby mica.
1)虎舌红组培条件为温度25±2℃,每天光照14h,光强1500~2000lux左右。
2)虎舌红组织培养快速繁殖的外植体以嫩叶(具有主叶脉)或顶芽或侧芽为好,最佳取材时间为3月中旬。
3)外植体消毒灭菌的有效方法是:先用肥皂水浸洗后,再用自来水冲洗1~2小时,冲洗干净后,晾干,切取其茎段、芽、嫩叶和叶柄分别放入装有75%酒精的烧杯中浸30s后取出,放入0.1%的升汞中消毒8min,在无菌条件下取出,用无菌水冲洗4~6次,为了冲洗掉残留的(Hg~(2+)),每次无菌水冲洗时间不少于2分钟,并不停地振荡,以便无菌水与材料充分接触。接种时,用干净滤纸吸干外植体表面水分,可以明显减少污染率和褐变率。
4)初代培养:芽萌发的最佳培养基为:2/3MS+BA2mg/L+IBA0.2mg/L+蔗糖3%,萌发率为91.0%;愈伤组织诱导的最佳培养基为MS+BA1.0mg/L+2,4-D1.0mg/L+蔗糖3%或MS+BA0.2mg/L+NAA0.2mg/L+2,4-D0.5mg/L+蔗糖3%,诱导效果较好,愈伤组织诱导率分别为75.19%,67.72%。
5)继代培养:芽苗增殖最佳培养基为MS+BA1.5mg/L+NAA0.1mg/L+蔗糖3%,增殖系数可达6.6,且芽苗生长良好。
6)生根培养:生根培养基以1/2MS+IBA0.5mg/L+NAA0.5mg/L+蔗糖2%为好,生根率达93.6%。在此培养基上添加不同浓度的活性炭,以0.2%AC效果更好。
7)炼苗:在基质选择上,珍珠岩与蛭石1:1混和炼苗成活率最高(64.4%),腐殖质土次之(53.3%),而纯砂最差(35%)。
8)试验结果按最佳处理计算,繁殖系数以30~40天左右为一个增殖周期,增殖系数为6~7,年理论增殖倍数可达2.8×10~8,能够在短期内达到大量增殖的目的。
Studies were carried out to find out the best composition of medium and propagation procedure by using the explants of terminal buds, axillary's buds, leaves of Ardisia Mamillata Hance. The results were as follows:
1)Culture conditions: temperature 25 2 , 14 hours illumination every day, and about 1500 Lux illumination intensity.
2)The optimal explants were young leaves (with partial main vein), shoot tips of terminal buds or lateral buds in middle March.
3)Effective surface sterilization of the primary explants was to soak them in 0.1% mercuric chloride for 8 minutes after washed in tap water for 1 ~2 hours and sterilized in 75% alcohol for 30 secends. Bloting the cultured material could prevent browning effectively when inoculating it on callus-inducing culture medium.
4)Primary cultivation: The best medium for bud's sprouting in initiation culture was 2/3MS+BA2mg/L+IBA0.2 mg/L in which sprouting rate could reach 91%. The best Callus-inducing culture medium was MS+BAlmg/L+2,4-D1.0mg/L or MS+ BA0.2mg/L +NAA0.2 mg/L +2, 4-D 0.5mg/L. Callus-inducing rate were 75.19% and 67.72% respectively.
5)The best subculture medium was MS+BA1.5mg/L+NAA0.1 mg/L+sucrose3%.
Where the multiplication rate was 6.6 or 2.8 108 per year.
6)The best rooting medium was l/2MS+IBA0.5mg/L+NAA0.5 mg/L +sugar2% +0.2%AC. Where the rooting rate could reach 93.6%.
7)Training seedling: The survial rate could reach 64.4% when the hardened rooted test tube plants were transplanted into the medium with 1/2 vermiculite and 1/2 ruby mica.
引文
[1]珍稀观叶植物——虎舌红.资源开发与市场,2003(2)
[2]一种长年置于室内的珍稀观叶植物——虎舌红.农业科技与信息,2000(6)18
[3]陈正华.木本植物组织培养及应用.高等教育出版社.1986
[4]惠长敏、韩宣等.花卉繁种的问题.北方园艺。1996(4):33
[5]谭文澄、戴策刚.观赏植物组织培养技术.中国林业出版社.1991
[6]邵宏波、初立业.花卉园艺植物快速繁殖研究现状(1).植物杂志.1994
[7]张涛、于永亮 花卉组织培养概况.河北林学院学报.1994(4):358
[8]朱西儒.从生物工程认识植物保护研究的发展趋势.生物技术通报.1997
[9]阙国宁,张健如.组培苗商品化:现状与对策.林业科技开发,1996,10(3):3~5
[10]王祥初.观果新贵——虎舌红.园林,2001
[11]中国植物志.第15卷(82~84)
[12]禹玉华.花卉新秀——虎舌红.农村经济与科技,2001,12(111)
[13]王意成.中国花经:471~472
[15]江香梅,邓小梅.虎舌红的组织培养和植株再生.
[16]卢其能.虎舌红的生物学特性与组织培养研究.江西林业科技,2002,1
[17]曹效东,曹孜义.植物试管繁殖的成本与效益浅析.植物生理学通讯,1996,32(4):284~291)
[18]王小菁,李玲.植物生长调节剂在植物组织培养中的应用.化学工业出版社.
[19]高亦珂,赵勃等.菊花茎叶外植体再生体系的研究.北京林业大学学报,2001,23(1):32~33
[20]李燕.虎舌红的繁殖.特种经济动植物.2002,5(8)
[21]虎舌红模式化栽培通过江西省科技鉴定验收,江西林业科技,2002(2)27
[22]室内珍稀植物虎舌红.中国花卉园艺,2001
[23]倪德祥,冯文煦等.一品红花轴培养成完整植株.植物生理学通报,1986,(3):46~57
[24]Ballester A,Sanchez M.C et al. Etiolationas a pretreatment for in vitro establishment and multiplication of mature Chestnut. Physiol plant, 1989,7:395~400
[25]南京农业大学编.田间试验和统计方法.北京:农业出版社,1994
[26]周纪芗.实用回归分析方法.上海:上海科学技术出版社,1990
[27]明道绪主编.生物统计附试验设计.中国农业出版社,2002年6月
[28]周俊彦,郭扶兴.植物快速营养繁殖中繁殖速度及产率的计算.植物学通报,1991,8(2):60~63
[29]卢纹岱,朱一力等.统计分析软件SPSS for Windows从入门到精通.电子工业出版社,1997年6月.
[30]白宝璋,田纪春等.植物生理学.中国农业科技出版社,1996
[31]余新大,张国富等.细胞工程.科学普及出版社,1988,21~22
[32]苏秀城,余小涵等.杉木优良无性系组培繁育试验.福建林业科技,1997,24,(4):36~40
[33]谢耀坚.桉树组织培养研究进展.世界林业科技,2000,13(6):14~19
[34]杨乃博.几种木本植物的组织培养及器官发生.植物生理学通讯,1982(4):23~27
[35]王冬梅,黄学林.细胞分裂素类物质在植物组织培养中的作用机制.植物生理学通讯.1996,32(5):373~377
[36]南京林业大学.田间试验和统计方法.农业出版社,1994
[37]马庆虎,宋艳茹.植物激素的基因工程.植物学报.1993,35(4):318~328
[38]J.M.Bonga等,树木组织培养.中国林业出版社,1985
[39]潘远智,植物生长调节剂对花卉植物矮化效应研究,四川林业科技,2000,21(4):36~40
[40]田兴范,刘志强等.多效唑对菊花、蔓长春花试管苗生根的影响.园艺学报,1993,20(1):101~102
[41]李镜.几种名贵观赏植物的快速繁殖.河北农业大学学报,1997,20(1):30~36
[42]谷瑞升.植物离体培养器官发生调空机理的研究进展.
[43]王冬梅,黄学林等,细胞分裂素类物质在植物组织培养中的作用机制[J].植物生理学通讯,1996,(5):373-377.
[44]朱至清.花药和花粉培养.见:罗士伟、许智宏主编.经济植物组织培养.北京:科学出版社,1988,37
[45]王敬驹,匡柏健,曾慧.提高甘蔗组织培养效率的研究.植物学通报,1983,1(2):17
[46]颜昌敬编.植物组织培养手册.上海:上海科学技术出版社,1990
[47]费开韦,薛光荣.国外温带落叶果树组织培养研究综述.中国果树,1980(增刊)
[48]谭文澄,戴策刚.观赏植物组织培养技术.中国林业出版社,1991
[49]彭信海,宾秋实.植物组织培养在林木遗传育种的应用.经济林研究,1998,16(2):54~55
[50]沈效东等.生长调节剂对毛白杨叶愈伤组织诱导和植株再生的影响.宁夏农林科技,1996,(6):18~20
[51]李群,杜文平等.植物组织培养中控制与污染技术的研究.四川林业科技.1996,(20):22~24
[52]Ronse AC. In vitro propagation of Otacanthus cocruleus. Plant Cell.Tissue and organ Culture. 1992,30(3):243
[53]贾春兰,王纪方,杨建荣等.葡萄试管苗繁殖技术的研究.中国果树.1992(1):25
[54]Cronauer SS. Rernition of vegetative growth from aseptically cultured terminal floral apex of banana. Amer J Bd. 1985, 72(10):1598
[55]Berardi G. Micropropagation of callery pear from seeding explants. Sci Horticul(Amsterdam), 1993,53(1~2): 157
[56]Lee CH. Kim SB.Choi IM et al. Effect of growth regulator and medium composition on the growth of apple rootstock M.26. J of the Korean Soc for Horticul Sci, 1990,31(4):385
[57]Antonelli M. Chiariolli A. In vitro rooting of different peach genotypes. Acta Horticul 1988,227:414
[58]Wang QC. Factors affecting rooting of microcuttings of the pear rootstck Bp1O030.Sci Horticul, 1991, 45(3~4):209
[59]夏铭,吴降云,张丽梅.红豆杉组织培养中褐变问题的研究.生物技术.1996(3):18~20
[60]姚洪军,罗晓芳,田研亭.植物组织培养外植体褐变的研究进展.北京林业大学学报.1999(3):78~84
[61]董建华.几种热带水果的褐变与PPO.热带作物研究.1990(2):92~99
[62]罗士伟,许智宏.经济植物组织培养.北京科学出版社.1998
[63]崔澄,桂耀林.经济植物的组织培养与快速繁殖.北京:农业出版社.1985
[64]Mayer A M, Harel. Polyphenol Oxiduses in Plants. Phytochemistry. 1979(18): 193~195
[65]Dan-hua Yu, Carole P Mereclith, The influence of explant origin on tissue browing and shoot production in shoottip cultures of grapevine J. Amer. Soc. Hort. Sci. 1986(16):972~975
[2]一种长年置于室内的珍稀观叶植物——虎舌红.农业科技与信息,2000(6)18
[3]陈正华.木本植物组织培养及应用.高等教育出版社.1986
[4]惠长敏、韩宣等.花卉繁种的问题.北方园艺。1996(4):33
[5]谭文澄、戴策刚.观赏植物组织培养技术.中国林业出版社.1991
[6]邵宏波、初立业.花卉园艺植物快速繁殖研究现状(1).植物杂志.1994
[7]张涛、于永亮 花卉组织培养概况.河北林学院学报.1994(4):358
[8]朱西儒.从生物工程认识植物保护研究的发展趋势.生物技术通报.1997
[9]阙国宁,张健如.组培苗商品化:现状与对策.林业科技开发,1996,10(3):3~5
[10]王祥初.观果新贵——虎舌红.园林,2001
[11]中国植物志.第15卷(82~84)
[12]禹玉华.花卉新秀——虎舌红.农村经济与科技,2001,12(111)
[13]王意成.中国花经:471~472
[15]江香梅,邓小梅.虎舌红的组织培养和植株再生.
[16]卢其能.虎舌红的生物学特性与组织培养研究.江西林业科技,2002,1
[17]曹效东,曹孜义.植物试管繁殖的成本与效益浅析.植物生理学通讯,1996,32(4):284~291)
[18]王小菁,李玲.植物生长调节剂在植物组织培养中的应用.化学工业出版社.
[19]高亦珂,赵勃等.菊花茎叶外植体再生体系的研究.北京林业大学学报,2001,23(1):32~33
[20]李燕.虎舌红的繁殖.特种经济动植物.2002,5(8)
[21]虎舌红模式化栽培通过江西省科技鉴定验收,江西林业科技,2002(2)27
[22]室内珍稀植物虎舌红.中国花卉园艺,2001
[23]倪德祥,冯文煦等.一品红花轴培养成完整植株.植物生理学通报,1986,(3):46~57
[24]Ballester A,Sanchez M.C et al. Etiolationas a pretreatment for in vitro establishment and multiplication of mature Chestnut. Physiol plant, 1989,7:395~400
[25]南京农业大学编.田间试验和统计方法.北京:农业出版社,1994
[26]周纪芗.实用回归分析方法.上海:上海科学技术出版社,1990
[27]明道绪主编.生物统计附试验设计.中国农业出版社,2002年6月
[28]周俊彦,郭扶兴.植物快速营养繁殖中繁殖速度及产率的计算.植物学通报,1991,8(2):60~63
[29]卢纹岱,朱一力等.统计分析软件SPSS for Windows从入门到精通.电子工业出版社,1997年6月.
[30]白宝璋,田纪春等.植物生理学.中国农业科技出版社,1996
[31]余新大,张国富等.细胞工程.科学普及出版社,1988,21~22
[32]苏秀城,余小涵等.杉木优良无性系组培繁育试验.福建林业科技,1997,24,(4):36~40
[33]谢耀坚.桉树组织培养研究进展.世界林业科技,2000,13(6):14~19
[34]杨乃博.几种木本植物的组织培养及器官发生.植物生理学通讯,1982(4):23~27
[35]王冬梅,黄学林.细胞分裂素类物质在植物组织培养中的作用机制.植物生理学通讯.1996,32(5):373~377
[36]南京林业大学.田间试验和统计方法.农业出版社,1994
[37]马庆虎,宋艳茹.植物激素的基因工程.植物学报.1993,35(4):318~328
[38]J.M.Bonga等,树木组织培养.中国林业出版社,1985
[39]潘远智,植物生长调节剂对花卉植物矮化效应研究,四川林业科技,2000,21(4):36~40
[40]田兴范,刘志强等.多效唑对菊花、蔓长春花试管苗生根的影响.园艺学报,1993,20(1):101~102
[41]李镜.几种名贵观赏植物的快速繁殖.河北农业大学学报,1997,20(1):30~36
[42]谷瑞升.植物离体培养器官发生调空机理的研究进展.
[43]王冬梅,黄学林等,细胞分裂素类物质在植物组织培养中的作用机制[J].植物生理学通讯,1996,(5):373-377.
[44]朱至清.花药和花粉培养.见:罗士伟、许智宏主编.经济植物组织培养.北京:科学出版社,1988,37
[45]王敬驹,匡柏健,曾慧.提高甘蔗组织培养效率的研究.植物学通报,1983,1(2):17
[46]颜昌敬编.植物组织培养手册.上海:上海科学技术出版社,1990
[47]费开韦,薛光荣.国外温带落叶果树组织培养研究综述.中国果树,1980(增刊)
[48]谭文澄,戴策刚.观赏植物组织培养技术.中国林业出版社,1991
[49]彭信海,宾秋实.植物组织培养在林木遗传育种的应用.经济林研究,1998,16(2):54~55
[50]沈效东等.生长调节剂对毛白杨叶愈伤组织诱导和植株再生的影响.宁夏农林科技,1996,(6):18~20
[51]李群,杜文平等.植物组织培养中控制与污染技术的研究.四川林业科技.1996,(20):22~24
[52]Ronse AC. In vitro propagation of Otacanthus cocruleus. Plant Cell.Tissue and organ Culture. 1992,30(3):243
[53]贾春兰,王纪方,杨建荣等.葡萄试管苗繁殖技术的研究.中国果树.1992(1):25
[54]Cronauer SS. Rernition of vegetative growth from aseptically cultured terminal floral apex of banana. Amer J Bd. 1985, 72(10):1598
[55]Berardi G. Micropropagation of callery pear from seeding explants. Sci Horticul(Amsterdam), 1993,53(1~2): 157
[56]Lee CH. Kim SB.Choi IM et al. Effect of growth regulator and medium composition on the growth of apple rootstock M.26. J of the Korean Soc for Horticul Sci, 1990,31(4):385
[57]Antonelli M. Chiariolli A. In vitro rooting of different peach genotypes. Acta Horticul 1988,227:414
[58]Wang QC. Factors affecting rooting of microcuttings of the pear rootstck Bp1O030.Sci Horticul, 1991, 45(3~4):209
[59]夏铭,吴降云,张丽梅.红豆杉组织培养中褐变问题的研究.生物技术.1996(3):18~20
[60]姚洪军,罗晓芳,田研亭.植物组织培养外植体褐变的研究进展.北京林业大学学报.1999(3):78~84
[61]董建华.几种热带水果的褐变与PPO.热带作物研究.1990(2):92~99
[62]罗士伟,许智宏.经济植物组织培养.北京科学出版社.1998
[63]崔澄,桂耀林.经济植物的组织培养与快速繁殖.北京:农业出版社.1985
[64]Mayer A M, Harel. Polyphenol Oxiduses in Plants. Phytochemistry. 1979(18): 193~195
[65]Dan-hua Yu, Carole P Mereclith, The influence of explant origin on tissue browing and shoot production in shoottip cultures of grapevine J. Amer. Soc. Hort. Sci. 1986(16):972~975
© 2004-2018 中国地质图书馆版权所有 京ICP备05064691号 京公网安备11010802017129号 地址:北京市海淀区学院路29号 邮编:100083 电话:办公室:(+86 10)66554848;文献借阅、咨询服务、科技查新:66554700 |