浙江大学学报(农业与生命科学版)
浙江大學學報(農業與生命科學版)
절강대학학보(농업여생명과학판)
2013年
3期
274-280
,共7页
孔丹丹%阙亚伟%闫霞%李亚%陈卫良%王政逸*
孔丹丹%闕亞偉%閆霞%李亞%陳衛良%王政逸*
공단단%궐아위%염하%리아%진위량%왕정일*
水稻纹枯病菌%原生质体%制备%再生
水稻紋枯病菌%原生質體%製備%再生
수도문고병균%원생질체%제비%재생
Rhizoctonia solani%protoplast%preparation%regeneration
水稻纹枯病的病原菌是立枯丝核菌( Rhizoctonia solani Kühn),其病原菌( R . solani Kühn)又称为水稻纹枯病( rice sheath blight)菌,由立枯丝核菌侵染引起的水稻纹枯病是水稻上最重要的病害之一.为建立高效的水稻纹枯病菌原生质体制备技术体系,采用0.7 mol/L NaCl作为渗透稳定剂,对Glucanex、溶壁酶( lywallzyme)、纤维素酶(cellulase‐R‐10)、离析酶( macerozyme‐R‐10)、蜗牛酶( snailase)、崩溃酶( driselase)和裂解酶( lysing enzyme)等7种不同的胞壁裂解酶降解水稻纹枯病菌GD‐118菌株细胞壁的作用进行测定,并对不同酶组合及其酶质量浓度进行优化筛选.结果显示:Glucanex对水稻纹枯病菌细胞壁的降解效果最好,用20 mg/mL Glucanex处理1 g菌丝4 h后,可释放118畅5×104个原生质体;用15 mg/mL Glucanex和10 mg/mL lywallzyme混合酶处理,可高效降解水稻纹枯病菌细胞壁并获得大量原生质体,原生质体产量达3畅09×107个/g 菌丝,再生率达58%;Glucanex 和lywallzyme的混合酶对不同水稻纹枯病菌菌株的细胞壁降解和原生质体释放没有显著差异.可见,上述制备水稻纹枯病菌原生质体的方法具有较好的高效性和适用性,可满足该菌分子遗传研究的需要.
水稻紋枯病的病原菌是立枯絲覈菌( Rhizoctonia solani Kühn),其病原菌( R . solani Kühn)又稱為水稻紋枯病( rice sheath blight)菌,由立枯絲覈菌侵染引起的水稻紋枯病是水稻上最重要的病害之一.為建立高效的水稻紋枯病菌原生質體製備技術體繫,採用0.7 mol/L NaCl作為滲透穩定劑,對Glucanex、溶壁酶( lywallzyme)、纖維素酶(cellulase‐R‐10)、離析酶( macerozyme‐R‐10)、蝸牛酶( snailase)、崩潰酶( driselase)和裂解酶( lysing enzyme)等7種不同的胞壁裂解酶降解水稻紋枯病菌GD‐118菌株細胞壁的作用進行測定,併對不同酶組閤及其酶質量濃度進行優化篩選.結果顯示:Glucanex對水稻紋枯病菌細胞壁的降解效果最好,用20 mg/mL Glucanex處理1 g菌絲4 h後,可釋放118暢5×104箇原生質體;用15 mg/mL Glucanex和10 mg/mL lywallzyme混閤酶處理,可高效降解水稻紋枯病菌細胞壁併穫得大量原生質體,原生質體產量達3暢09×107箇/g 菌絲,再生率達58%;Glucanex 和lywallzyme的混閤酶對不同水稻紋枯病菌菌株的細胞壁降解和原生質體釋放沒有顯著差異.可見,上述製備水稻紋枯病菌原生質體的方法具有較好的高效性和適用性,可滿足該菌分子遺傳研究的需要.
수도문고병적병원균시립고사핵균( Rhizoctonia solani Kühn),기병원균( R . solani Kühn)우칭위수도문고병( rice sheath blight)균,유립고사핵균침염인기적수도문고병시수도상최중요적병해지일.위건립고효적수도문고병균원생질체제비기술체계,채용0.7 mol/L NaCl작위삼투은정제,대Glucanex、용벽매( lywallzyme)、섬유소매(cellulase‐R‐10)、리석매( macerozyme‐R‐10)、와우매( snailase)、붕궤매( driselase)화렬해매( lysing enzyme)등7충불동적포벽렬해매강해수도문고병균GD‐118균주세포벽적작용진행측정,병대불동매조합급기매질량농도진행우화사선.결과현시:Glucanex대수도문고병균세포벽적강해효과최호,용20 mg/mL Glucanex처리1 g균사4 h후,가석방118창5×104개원생질체;용15 mg/mL Glucanex화10 mg/mL lywallzyme혼합매처리,가고효강해수도문고병균세포벽병획득대량원생질체,원생질체산량체3창09×107개/g 균사,재생솔체58%;Glucanex 화lywallzyme적혼합매대불동수도문고병균균주적세포벽강해화원생질체석방몰유현저차이.가견,상술제비수도문고병균원생질체적방법구유교호적고효성화괄용성,가만족해균분자유전연구적수요.
Rice sheath blight caused by Rhizoctonia solani Kühn is one of the most important diseases on cultivated rice worldwide . Unlike most other fungal pathogens , R . solani forms heterokaryotic vegetative mycelia with multiple nuclei per hyphal cell and is unable to produce haploid asexual spores under normal conditions . These characteristics of R . solani may make it difficult to perform genetic transformation and functional analysis of genes . Production of large amount of protoplasts from this fungus is a prerequisite for the studies of molecular genetics , such as protoplast fusion and fungal transformation . Previously , some lytic enzymes and conditions for releasing R . solani protoplasts have been tested and optimized and several protocols for the preparation and regeneration of protoplasts from R .solani mycelium have been developed by some researchers . However , the efficiency of R .solani protoplasts releasing by these protocols is sometimes unstable due to different strains of R . solani or experimental conditions . Therefore , it is necessary to develop an efficient method for preparing protoplasts of rice sheath blight fungus .
@@@@The objectives of the present study were to evaluate various cell wall degradation enzymes and their combinations for releasing protoplasts from R . solani mycelium , and to develop an efficient protocol for yielding protoplasts .
@@@@Using 0.7 mol/L NaCl as stabilizer solution , seven different cell wall degradation enzymes , including Glucanex , lywallzyme , cellulase‐R‐10 , macerozyme‐R‐10 , snailase , driselase and lysing enzyme , and their combinations were evaluated for releasing protoplasts from R . solani GD‐118 mycelium which was harvested from potato dextrose liquid medium cultured at 28 ℃ for 36 h . The number of released protoplasts was counted by using haemocytometer under microscopy . The optimal concentration of lytic enzymes for the generation of protoplasts was determinated and the conditions to obtain and regenerate protoplasts of the fungus were also optimized .
@@@@Among the seven tested lytic enzymes , Glucanex was the most suitable enzyme for the digestion of R . solani GD‐118 cell wall . The protoplast yield in the treatment with 20 mg/mL Glucanex for 4 h was 23.7 × 104 cell/mL ( e . g . 118.5 × 104 cells per gram mycelium) . Moreover , the results showed that the optimal mixture enzymes of 15 mg/mL Glucanex and 10 mg/mL lywallzyme were effective in releasing protoplasts with the production of 3.09 × 107 protoplasts from per gram R . solani GD‐118 mycelium , and the obtained 58% protoplasts could be regenerated . In addition , the combination had similar effects on digesting cell wall of different strains of rice sheath blight fungus . Taken together , the mixture lytic enzymes of 15 mg/mL Glucanex and 10 mg/mL lywallzyme can effectively digest the cell wall of rice sheath blight fungus and produce abundant protoplasts .