溶磷菌对4种难溶性磷酸盐溶解能力的初步研究

以4种难溶性磷酸盐为培养基,发现供试菌株溶解这些磷酸盐的特性差异很大,真菌溶磷能力普遍比细菌要高得多。以NO3-为氮源时的溶磷量通常高于以NH4+为氮源时的溶磷量,只有2TCiF2对氟磷灰石及4TCiF6对磷酸铝的溶解能力以NH4+为氮源时较高。大多数菌株较易溶解CaP(氟磷灰石和磷矿粉),其次为AlP(AlPO4),而溶解FeP(FePO4·4H2O的能力都比较弱,只有曲霉2TCiF2具有较强的溶解FeP能力,尤其是当供给NO3-时,溶解FeP的活性比供给NH4+时大幅度提高。欧文氏菌4TCRi22和肠杆菌1TCRi15能大量地溶解氟磷灰石,而两株节杆菌对磷矿粉的溶解能力最强。供试菌株的溶磷作用可能是由于分泌的有机酸与金属离子络合或螯合作用所致,欧文氏菌和肠杆菌溶解难溶性磷过程中,非有机酸物质可能在起主要作用。     

石灰性土壤拉恩式溶磷细菌的筛选鉴定及溶磷特性

从山西石灰性土壤作物根际分离筛选出多株溶磷细菌,经过多次分离纯化得到一株溶磷能力较强的菌株W25,通过菌落形态、生理生化特性和16S rRNA序列分析,确定溶磷菌W25为拉恩式菌属.对W25溶解磷特性进一步研究表明:其对磷酸三钙、磷酸铝和磷酸铁最高溶磷能力分别为385.5、110.4、216.6 mg·L-1;在磷酸铝和磷酸铁培养液中,W25溶磷量与培养液pH的相关系数分别为0.56和0.81,呈极显著负相关;在不同碳氮源条件下,W25以葡萄糖为碳源和NH4NO3为氮源时对磷酸三钙的溶磷量最高,对碳源的利用顺序依次为葡萄糖＞乳糖＞蔗糖＞甘露醇＞淀粉,对氮源的利用顺序依次为NH4NO3 ＞NH4Cl＞(NH4)2SO4＞NaNO3＞KNO3.不同氮源对W25产生有机酸的种类影响较大,以铵态氮为氮源产生甲酸和乙酸,以硝态氮为氮源产生草酸和琥珀酸,以硝酸铵为氮源还产生柠檬酸.     

铁尾矿区油松根际溶磷泛菌D2的筛选鉴定及溶磷特性

从河北省迁安市马兰庄镇铁尾矿植被恢复区油松根际分离出2株溶磷细菌,经过平板初筛和摇瓶复筛得到1株溶磷能力较强的菌株D2.通过菌落形态、生理生化特性及16S rDNA序列分析,确定此菌株D2属于泛菌属.利用液体发酵试验测定不同碳源、氮源对菌株D2溶磷能力的影响,通过高效液相色谱测定D2在不同氮源条件下产生有机酸的种类和浓度.结果表明:菌株D2对磷酸三钙有较强的溶磷能力,培养液有效磷含量最高为392.13 mg·L^-1,菌株D2的溶磷能力在碳源为葡萄糖、氮源为硫酸铵时效果最好;高效液相色谱测定发现,不同氮源条件下,D2分泌有机酸的种类和浓度存在差异,以硫酸铵、氯化铵、硝酸钾、硝酸钠、硝酸铵为氮源,均产生草酸、甲酸、乙酸和柠檬酸,以硫酸铵、氯化铵、硝酸铵为氮源还产生苹果酸.相关性分析表明,乙酸含量与有效磷含量间呈显著正相关(r=0.886,P<0.05),表明溶磷泛菌D2分泌的乙酸对无机磷的溶解有明显的促进作用,这也很可能是该菌株的重要溶磷机制之一.     

溶磷菌和固氮菌溶解磷矿粉时的互作效应

采用4株溶磷菌（Lx81、Dm84、Jm92、Lx191）、和3株固氮菌（ChW5、ChW6、ChO6）单独和混合接种后测定培养液有效磷含量、pH值及总有机酸含量的方法,研究溶磷菌和固氮菌溶解磷矿粉时的互作效应。结果表明,相对于单独接种溶磷菌：Lx81与3株固氮菌分别混合培养能提高磷矿粉的溶解能力,4株溶磷菌与ChW6,Lx81、Dm84、Lx191与Ch06分别混合培养及Jm92＋ChW5组合溶磷量极显著增加（P〈0．01）;Dm84＋ChW5、Lxl91＋ChW5、Jm92＋Ch06组合的溶磷量下降（P〈0．01）。除Lx81＋ChW6、Lx81＋Ch06培养液pH值降低外,混合培养的其它组合培养液pH值均较单独接种溶磷菌时升高。有机酸测定结果表明,Lx81、Jm92与ChW5、Ch06分别混合培养、ChW6＋Lx81组合有机酸含量升高（P〈0．01）,其它7种组合的有机酸含量均较单独接种溶磷菌的值下降（P〈0．01）。溶磷菌和固氮菌单菌培养时溶磷量与pH值、溶磷量与总有机酸含量及pH值与总有机酸含量之间呈现线性相关;Dm84、Lx191与3株固氮菌分别混合培养溶磷量与pH值之间、Lx81与3株固氮菌分别混合培养溶磷量与总有机酸含量之间呈现线性相关,其它组合的溶磷量与pH值、总有机酸含量间没有相关性。溶磷菌和固氮菌混合培养对溶解磷矿粉既有协同作用也有拮抗作用。     

出芽短梗霉F4的溶磷能力及机理

从安徽省铜陵市铜官山尾矿库木贼根际分离筛选出的出芽短梗霉F4,以磷酸钙、磷酸铝、磷酸铁和磷矿粉4种不同磷源进行液体培养,测定培养液的pH、水溶性磷、菌体磷及有机酸含量.结果表明： 菌株F4对不同磷源的溶磷能力为：磷酸铝>磷酸铁、磷酸钙>磷矿粉,溶磷量均高于200 mg·L^-1;培养液pH在48 h内迅速下降,以磷酸铝、磷酸铁为磷源的培养液pH下降幅度明显大于磷酸钙与磷矿粉.出芽短梗霉F4产生的有机酸主要为草酸、柠檬酸和酒石酸,其中,以草酸为主.菌株的溶磷能力与有机酸无显著相关性,而与pH呈显著相关.接种出芽短梗霉F4时加入葡萄糖,尾矿中速效磷含量显著增加,说明出芽短梗霉F4在尾矿生态修复中具有潜在的应用价值.
     

不同碳源对三种溶磷真菌溶解磷矿粉能力的影响

通过液体培养法 ,对 3种溶磷真菌利用葡萄糖、果糖、蔗糖、麦芽糖、淀粉和纤维素等碳源溶解宜昌产磷矿粉的试验 ,结果表明 ,菌株P2 3在供给葡萄糖时的溶磷能力最高 ,并在一定程度上能够利用长链碳源淀粉和纤维素为营养而溶磷 ;而高效溶磷菌株P6 6和P39溶磷的最佳碳源是果糖和麦芽糖 ,该两菌株利用淀粉和纤维素的溶磷效果很小 ,甚至不溶磷。 3种溶磷真菌培养滤液 pH值、可滴定酸含量与其溶磷量之间的相关性因菌株而异 ,差别很大。菌株P2 3培养滤液pH值、可滴定酸含量与其溶磷量之间相关性很低 ,但菌株P6 6和P39培养滤液pH值、可滴定酸含量与其溶磷量之间相关性却达到极显著水平 (P <0 0 1)。结果表明 ,不同碳源对溶磷菌溶解磷矿粉能力影响很大 ,分析推断 3种菌株产生的有机酸活化磷矿粉能力为P6 6>P39>P2 3。     

一株溶磷真菌筛选鉴定及其溶磷促生效果

【目的】从高产农田筛选高效溶磷微生物菌株,为溶磷微生物肥料开发提供高效菌种资源。【方法】利用菌株的形态学特性、培养特征和ITS rDNA序列分析方法进行菌株鉴定,结合液体培养和土壤培养方法研究菌株的溶磷能力,进而采用温室盆栽和田间小区试验,明确溶磷菌P83促进作物生长和提高作物产量的作用效果。【结果】溶磷菌株P83鉴定为斜卧青霉菌(Penicillium decumbens)。液体条件下培养10 d,菌株P83表现显著高效的溶磷能力,对Ca3(PO4)2(5g/L)的溶解效果,有效磷达956 mg/L,溶解率为42.68%,对湖南永和磷矿粉的溶液效果,有效磷达到152.8 mg/L;将P83菌株分别接种于施用Ca3(PO4)2、Zn3(PO4)2和磷矿粉(RP)3种磷源的盆栽试验土壤中,结果显示,菌株P83对玉米植株促生效果比对照显著提高,玉米植株鲜重提高9.5%-89.2%、干重增加35%-231%,土壤有效磷提高2.1-40.5 mg/kg。田间小区玉米产量结果显示,溶磷菌P83增产效果最好(P=0.05),玉米子粒产量达9.2t/hm2,比不接种菌剂的对照增加2.4 t/hm2,增产率为35.3%。【结论】获得了一株溶解难溶磷的斜卧青霉菌P83,它能够活化多种难溶磷、显著增加土壤有效磷水平,对玉米生长和增加作物产量具有显著作用,是一株展现良好应用前景的高效溶磷菌种。     

一株耐盐日本曲霉的筛选及其溶磷促生作用

【目的】从内蒙古种植葵花的盐碱地中筛选高效溶磷真菌,为盐碱地增产节肥开发生物肥料提供溶磷菌种资源。【方法】利用ITS r DNA序列鉴定菌株、固体培养基测定耐盐性,液体摇床培养与盆栽试验结合分析菌株溶磷能力,盆栽和田间试验明确菌株M1促进作物生长和增产作用;LC-MS技术测定菌株M1在液体培养基中分泌有机酸和植物激素含量,明确菌株M1的溶磷和促生机理。【结果】溶磷菌株M1鉴定为日本曲霉(Aspergillus japonicus)。液体培养基接种菌株M1培养6 d,以Ca_3(PO_4)_2为磷源时上清液有效磷达1020.89 mg/L,溶解率为63.30%;以AlPO_4为磷源时有效磷达995.69 mg/L,溶解率为48.59%;以贵州开阳磷矿粉、江苏锦屏磷矿粉、云南晋宁磷矿粉、河北钒山磷矿粉和云南昆阳磷矿粉为磷源接种菌株M1,从晋宁磷矿粉释放的有效磷浓度最高,达到363.64 mg/L。菌株M1可耐受10%NaCl。将M1制备的菌剂分别接种于施用Ca_3(PO_4)_2、AlPO_4和开阳磷矿粉3种磷源的4种盆栽试验土壤包括北京石灰性潮土、安徽黏性潮土、安徽水稻土和山东沿海盐潮土。结果显示,菌株M1对玉米植株促生效果显著,玉米植株鲜重比对照提高2.14%–90.91%、干重增加22.15%–268.28%;土壤有效磷提高21.81–24.27 mg/kg。菌株M1与4种土壤的适配性均高于对照菌株DSM 821。田间小区花生产量结果显示,接种溶磷菌剂M1增产效果最好,花生果实产量达4.46 t/hm~2,比不接种菌剂的对照处理增加0.81 t/hm~2,增产22.19%。菌株M1在含有磷酸三钙、磷酸铝和开阳磷矿粉3种难溶磷培养液中经过6 d培养,均产生7种有机酸,其中草酸和柠檬酸含量最高,分别为616.16 mg/L和413.69 mg/L;培养液均能检测到吲哚乙酸(IAA)和玉米素,IAA含量为15.45–77.58 mg/L,玉米素浓度为0.06–0.11 mg/L。【结论】获得了一株高效溶解多种难溶磷的日本曲霉菌M1,它能显著增加土壤有效磷、促进玉米生长和花生增产,与4种典型土壤适配性好,具有良好的农业应用前景。     

两株溶磷真菌的筛选、鉴定及溶磷效果的评价

【目的】从作物根围土壤中筛选高效溶磷菌株。【方法】结合溶磷圈筛选法和钼锑抗比色法评价菌株的溶磷能力;利用菌株的形态学特性、培养性状和微管蛋白β-tubulin基因序列分析方法进行菌株的鉴定;采用气相色谱-质谱法(GC-MS)对溶磷菌的产酸物质进行分析;并用平板亲和性实验测定菌株间的兼容性。【结果】筛选得到2株高效溶磷菌株P1-1、P2-2;经鉴定,菌株P1-1为黑曲霉(Aspergillus niger),P2-2为塔宾曲霉(A.tubingensis)。2株溶磷菌株的产酸物质相同,均为草酸、葡萄糖酸、乳酸和甘油酸。这2株溶磷菌与杀线虫功能菌株淡紫拟青霉(Purpureocillium lilacinum)、橄榄色链霉菌(Streptomyces olivaceus)和苍白杆菌(Ochrobactrum pseudogrignonense)兼容性好。2菌株分别在Ca_3(PO_4)_2、Zn_3(PO_4)_2、羟基磷灰石为磷源的无机磷固体培养基中25°C培养5 d,测定溶磷圈的直径(D)与菌落直径(d),通过计算其比值D/d的大小对比,以及在Ca_3(PO_4)_2、Zn_3(PO_4)_2、羟基磷灰石为磷源的液体培养基中培养5 d,测定发酵液中有效磷含量进行比较后判定,这2株溶磷菌溶解磷的能力强且效果相当。【结论】获得了2株高效的溶磷真菌。它们能活化多种难溶性磷源,同时伴随挥发性酸性物质的产生;2个菌株与1组杀根结线虫微生物菌群兼容性均良好。     

红树林溶磷菌的初步鉴定、溶磷能力测定及其优化培养

对分离来自华南红树林的溶磷菌进行16S rDNA或ITS等基因水平上的初步鉴定, 测定其溶解无机磷的能力, 并对溶磷菌的生长培养基条件进行优化。结果表明, 溶磷真菌的溶磷效果明显强于溶磷细菌, 且溶磷真菌的溶解无机磷能力与培养液的pH呈极显著负相关, 而溶磷细菌的溶磷能力与pH没显著相关关系。单因素实验表明, 对供试菌株生长的合适碳源为麦芽糖, 氮源为尿素。通过正交实验得到的优化培养基为麦芽糖5 g/L、尿素0.05 g/L、NaCl 5 g/L、pH 5, 在30°C下培养48 h菌落总数可达6.06×     

荧光假单胞菌CLW17菌株pqqE和GDH基因的功能

[背景]磷是植物生长所必需的大量元素,但绝大多数不能被植物吸收利用。然而溶磷微生物能够分泌有机酸来溶解土壤中难溶性磷,提高土壤中磷的利用率,促进植物生长,提高作物的产量和品质。[目的]探究高效解磷荧光假单胞菌CLW17菌株的pqqE和GDH基因的生理学功能。[方法]利用生物在线软件对2个基因编码蛋白进行生物信息学分析。利用同源重组技术分别获得pqqE和GDH基因缺失突变株(CLW17ΔpqqE,CLW17ΔGDH),并使用接合转移的方式获得回补菌株(ΔpqqE/pqqE,ΔGDH/GDH)。分别采用NBRIP培养基、钼锑抗比色法及高压液相色谱法(HPLC)对野生型、突变株及互补株的溶磷及产有机酸能力进行检测。[结果]pqqE和GDH基因编码氨基酸数目分别为390和803,均无信号肽。pqqE无跨膜结构域,而GDH预测有5个跨膜结构域。pqqE和GDH基因是CLW17菌株的溶磷相关基因,2个基因的缺失均使该菌株的溶磷能力显著下降,而回补株可以恢复溶磷能力。CLW17野生株能分泌多种有机酸,其中葡萄糖酸(gluconic acid,GA)含量最多,其次是乙酸;但敲除株产有机酸的能力明显降低...     

草酸青霉YTY及其突变体解磷能力、pH和分泌有机酸的关系

本研究利用离子束-UV复合诱变草酸青霉YTY选育高效解磷突变体,分析了出发菌株YTY及其突变体解磷过程中的解磷能力、pH和有机酸的变化及其相关性,探讨草酸青霉的解磷机理。结果表明: 离子束-UV复合诱变选育获得5株高效解磷突变株P9-8、P9-9、P15-4、P15-6和P15-7,解磷能力均较YTY提高60%以上。解磷过程中突变株解磷能力及解磷速率均高于YTY,而pH显著低于YTY,同时,突变体分泌有机酸种类及含量发生了不同程度的变化,突变体和YTY均可分泌乳酸、乙酸和草酸,P9-8还产生了柠檬酸。皮尔逊相关分析显示,YTY及5株突变株的解磷能力和pH值呈显著负相关;YTY及其突变体(P15-4除外)的解磷能力与有机酸浓度和pH呈显著相关。分泌有机酸和降低环境pH值可能是草酸青霉解磷的内在机制,离子束-UV复合诱变可引起草酸青霉YTY有机酸分泌种类和分泌量的变化,还可能诱发YTY启动其他H⁺释放途径降低pH参与解磷。本研究为高效解磷青霉的开发及青霉解磷机理阐明提供了生物材料及理论依据。     

杨树根际解无机磷细菌Mp1-Ha4的鉴定及其解磷机理

解无机磷细菌能够溶解土壤中的难溶性磷酸盐,增加土壤有效磷含量,促进植物生长。以一株杨树根际土壤中筛选得到的解无机磷细菌Mp1-Ha4为研究对象,利用分子生物学的方法对该菌株进行鉴定,测定了其对磷酸钙、磷酸铝和磷酸铁的解磷能力,并对该菌株9 d内的磷酸钙溶解动力学进行了研究。结果表明,解无机磷细菌Mp1-Ha4为一株西地西菌Cedecea sp.,其对磷酸钙的溶解能力远强于对磷酸铝和磷酸铁的溶解能力。在NBRIP液体培养基中,该菌株对磷酸钙的溶解能力达到了497.4 mg/L,在其对磷酸钙解磷过程中,培养基pH及可滴定酸度与解磷量分别呈显著负、正相关。高效液相色谱分析显示,该菌株在解磷过程中分泌了大量有机酸,主要包括α-酮戊二酸,酒石酸和苹果酸。分泌有机酸,降低环境pH可能是解无机磷细菌西地西菌(Cedecea sp.)Mp1-Ha4溶解难溶性磷酸盐的主要机制,同时该菌株对磷酸钙的高效溶解作用使其具有较大的研究和应用前景。     

黑曲霉解磷能力的影响因素及培养条件优化

本文探讨了培养条件下黑曲霉解磷能力的主要影响因素。通过单孢株筛选得到解磷能力较强的菌株Xj-2,其在液体培养基中的解磷能力达到539.90 mg·L^-1。解磷发酵动力学模型模拟发现,其解磷能力在培养的第4 天达到平稳,可作为终止发酵时间。不同磷源培养液中菌株Xj-2的解磷量依次为磷酸钙(539.90 mg·L^-1)>磷酸锌(238.45 mg·L^-1)>磷酸铁(182.64 mg·L^-1)>磷矿粉(71.80 mg·L^-1)>磷酸铝(24.40 mg·L^-1)。通过单因素试验并结合响应面优化,研究了其解磷最佳条件。结果表明: 碳源对Xj-2的解磷能力影响最大,其次是菌群密度和培养液pH。当培养温度35 ℃、转速160 r·min^-1、培养液pH 6.0、氮源(尿素)浓度0.79 g·L^-1、碳源(葡萄糖)浓度10.00 g·L^-1、菌群密度3.8%、培养时间为4 d时,Xj-2的解磷能力最高,为616.81 mg·L^-1。     

拉恩氏菌W25对缓冲容量的响应及其产酸特性

【目的】进一步了解拉恩氏菌W25的溶磷机理和对土壤缓冲容量的响应。【方法】在液体摇瓶培养过程中,采用调节培养液pH的方法研究模拟土壤的缓冲容量对拉恩氏菌W25溶磷量的影响;通过单因子试验和HPLC相结合的方法,研究不同碳源、磷源条件下W25的溶磷能力及产酸特性。【结果】拉恩氏菌W25在磷酸三钙培养液中培养120 h后有效磷含量达到最大值,培养液有效磷含量与培养液pH变化之间呈极显著负相关性(P<0.01);W25在培养第48?96 h具有较强的缓冲能力,培养液有效磷含量加碱处理与未加碱处理差异不显著(P<0.05),从第120 h开始,缓冲能力开始减弱,在168 h后基本丧失了缓冲能力;W25在不同碳源条件下溶磷能力差异显著(P<0.05),依次为葡萄糖>乳糖>蔗糖>甘露醇>淀粉,不同磷源中培养液有效磷含量差异极显著(P<0.01),依次为磷酸三钙>磷酸铁>磷酸铝>磷矿粉;不同碳源、磷源条件下W25培养液中有机酸的种类和浓度差异较大,W25溶磷能力的大小不仅与产酸的种类有关,而且也与产酸的浓度有关。【结论】研究结果为更深入研究拉恩氏菌溶磷机理提供条件,为拉恩氏菌的应用提供理论基础。     

Interactions of an acid tolerant strain of phosphate solubilizing bacteria with a few acid tolerant crops

Phosphate solubilizing bacteria (PSB) were isolated from sixty soil samples of various soil classes and cropping histories in Himalayan regions of Uttar Pradesh, India by enrichment culture techniques. Phosphate solubilization and acid tolerance of each strain was estimated. A strain (PAS-2) isolated froma pasture and waste land of pH 4.8, organic matter 2.6% available N 265kg ha^-1, available P₂O₅(Bray's II) 2.3kg ha^-1 and available K₂O 353 kg ha^-1 had the highest P-solubilization (45 µg P per mL per day) and also highest acid tolerance rating 42. The strain was identified as Bacillus sp. Seed inoculation of this bacterial strain resulted in significant increases in grain and vegetative yield of fingermillet (Elosine coracana), maize (Zea mays), amaranth (Amaranthus hypochondriacus), buckwheat (Fagopyrium esculentum), frenchbean (Phaseolus vulgaris) with or without added P sources. The significant grain yield (quintol ha^-1) with phosphate and seed inoculation ranged from 33.85 in maize, 26.33 in frenchbean, 22.41 in buckwheat, 20.71 in amaranth and 19.19 in fingermillet as compared to controls. The highest response was observed with frenchbean followed by fingermillet, buckwheat, amaranth and maize. Phosphate use efficiency was highest in frenchbean followed by maize and lowest and almost at par in buckwheat, amaranth and fingermillet. Available phosphate was also highest in frenchbean cultivated plot followed by amaranth, fingermillet, buckwheat and maize. The MPN count of phosphate solubilizing bacteria were also influenced by seed inoculation of strain PAS-2. Frenchbean exerted greaterrhizosphere effect followed by pseudocereals and cereals. Likewise, phosphate nutrition of crops were also improved through seed inoculation irrespective of added P sources. The study thus demonstrated that selection of efficient strain of PSB from acid soil and its seed inoculation in selected crop genotype is beneficial in boosting up crop yield in low productive hill soil. Seed inoculation also created greater rhizosphere effect over uninoculation which improved P-nutrition of crops and also available soil P.     

Role of soil microorganisms in improving P nutrition of plants

Phosphorus (P) is one of the major plant growth-limiting nutrients although it is abundant in soils in both inorganic and organic forms. Phosphate solubilizing micro-organisms (PSMs) are ubiquitous in soils and could play an important role in supplying P to plants in a more environmentally friendly and sustainable manner. Although solubilization of P compounds by microbes is very common under laboratory conditions, results in the field have been highly variable. This variability has hampered the large-scale use of PSMs in agriculture. Many reasons have been suggested for this variability, but none of them have been extensively investigated. In spite of the importance of PSMs in agriculture, the detailed biochemical and molecular mechanisms of P solubilization are not known. Recent work in our laboratory has shown that the conditions employed to isolate PSMs do not reflect soil conditions and that PSMs capable of effectively releasing P from soil are not so highly abundant as was suggested in earlier studies. These studies have also indicated that the mineral phosphate solubilizing (mps) ability of microbes could be linked to specific genes, and that these genes are present even in non P solubilizing bacteria. Understanding the genetic basis of P solubilization could help in transforming more rhizosphere-competent bacteria into PSMs. Further research should also focus on the microbial solubilization of iron (Fe) and aluminum (Al) phosphates, as well as mobilization of the organic phosphate reserves present in the soils.     

Identification,characterization and optimization of phosphate solubilizing rhizobacteria (PSRB) from rice rhizosphere

Two billion people worldwide take rice (Oryza sativa L.) as a staple food. Phosphorus (P) and Nitrogen (N) are the major requirements of rice; although these are available in limited concentrations within rice growing regions. Among different types of Plant growth-promoting rhizobacteria (PGPR), Phosphate solubilizing rhizobacteria (PSRB) constitute an important class. These are known for plant growth promotion by enhancing P and N uptake. PSRB are nowadays used as biofertilizers to restore the soil health. Under the present investigation identification, characterization and optimization of phosphate solubilizing activity of these microbes at different pH, temperature and salt concentrations was carried out. Thirty-seven isolates were recovered from different regions of rice rhizosphere on Pikovskaya (PVK) agar among which 15 isolates were recovered from R.S. Pura, 12 isolates from Bishnah and 10 isolates were recovered from Akhnoor sector of Jammu, India. A prominent halo zone of clearance was developed around the colonies of 12 different isolates, indicating phosphate solubilization activity. Four distinct isolates were amplified, cloned and sequenced for taxonomic identification using 16S primers. The results indicated that PS 1, PS 2, PS 3, PS 4 were related to Pseudomonas aeruginosa, Bacillus subtilis strain 1, B. subtilis strain 2, B. subtilis strain 3, respectively. These strains when grown at a wide range of ecological factors showed maximum growth at pH between 6.8 and 8.8, temperature between 28 °C and 37 °C and salinity between 1% and 2%. Screening for phosphate solubilization activity revealed that the halo zone diameter formed by these isolates extended from 2.1 to 3.2 mm. The phosphate solubilizing efficiency (SE) ranged from 35.4 to 50.9 with highest value of 50.9 by PS4 and maximum P solubilization of 10.22 µg/ml was recorded by PS4 at 7th day. Phosphate solubilization activity of these identified PSRB strains can be utilized and explored in the rice growing belts of Jammu region which are deficient in phosphorus. MIC value for zinc sulphate heptahydrate in 12 isolates varied from 1 mg/ml to 6 mg/ml. Phosphate solubilization activity and MIC of these identified PSRB strains can be utilized and explored in the rice growing belts of Jammu region which are deficient in phosphorus.     

一株高效解磷肠膜明串珠菌的分离鉴定及解磷能力研究

【背景】植物根际土壤含有多种溶磷微生物,但是具有溶磷能力的肠膜明串珠菌未见报道。【目的】从脐橙根际土壤分离高效解磷菌,研究其解磷应用。【方法】通过初筛和复筛从23株菌中筛选解磷能力较强的菌株,同时采用钼蓝比色法测定磷含量。通过测定发酵液中小分子有机酸含量、磷酸酯酶酶活及pH值的变化,探究菌株的解磷机理。【结果】经过筛选得到9株具有一定解磷能力的菌株。通过菌种16S rRNA基因序列分析和生理生化实验确定其中一株菌为肠膜明串珠菌,命名为肠膜明串珠菌G7。培养基初始pH6.0、碳源为葡萄糖、氮源为硫酸铵时G7的解磷能力较佳。G7发酵过程中产生大量有机酸,而其酸性磷酸酯酶活性高于碱性磷酸酯酶。【结论】碳源、氮源以及初始pH值都能影响G7的解磷能力,其解磷能力主要缘于在发酵过程中产生了大量小分子有机酸,关于G7的解磷机理还需要更深入的研究。     

Organic Acid Secretion and Phosphate Solubilizing Efficiency of Pseudomonas sp. PSB12: Effects of Phosphorus Forms and Carbon Sources

Secretion of organic acids is an important mechanism for phosphate solubilizing bacteria (PSB) to dissolve insoluble phosphorus in soil. However, the composition of organic acids produced by PSB in the presence of different phosphorus compounds is poorly known, and little is known about the ability of PSB to degrade pollutants in sediment. In this study, we isolated a strain Pseudomonas sp. PSB12 from the sediment of the Qihe River. PSB12 had maximum phosphate solubilization index (SI) of 3.86 on Pikovskaya's agar medium. The phosphate solubilizing activity was associated with the release of organic acids produced from glucose, while the composition of organic acids produced by PSB12 was dependent on the phosphorus forms. When initial soluble phosphorus was insufficient (in MP1 and MP2 media), gluconic acid was the predominant organic acid. In contrast, formic acid, butyrate, and propanedioic acid were the main organic acids produced when only soluble phosphorus (MP3) was supplied. RT-PCR indicated that the expression of glucose dehydrogenase gene (gcd) of PSB12 was two- to four-fold higher in MP1 than in MP3. PSB12 also possessed the phenol hydroxylase gene (phe) suggesting that phenol could be used as the carbon source to dissolve insoluble phosphorus. PSB12 is a potential candidate for in situ bioremediation and for promoting plant growth in soil contaminated by phenol with low levels of soluble phosphorus.