CN100529051C - Method for preparing endophyte of plant - Google Patents

Method for preparing endophyte of plant Download PDF

Info

Publication number
CN100529051C
CN100529051C CNB2007100657244A CN200710065724A CN100529051C CN 100529051 C CN100529051 C CN 100529051C CN B2007100657244 A CNB2007100657244 A CN B2007100657244A CN 200710065724 A CN200710065724 A CN 200710065724A CN 100529051 C CN100529051 C CN 100529051C
Authority
CN
China
Prior art keywords
plant
endophyte
supernatant liquor
final concentration
preparing
Prior art date
Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
Expired - Fee Related
Application number
CNB2007100657244A
Other languages
Chinese (zh)
Other versions
CN101050424A (en
Inventor
王浩鑫
曾英
沈月毛
Current Assignee (The listed assignees may be inaccurate. Google has not performed a legal analysis and makes no representation or warranty as to the accuracy of the list.)
Kunming Institute of Botany of CAS
Original Assignee
Kunming Institute of Botany of CAS
Priority date (The priority date is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the date listed.)
Filing date
Publication date
Application filed by Kunming Institute of Botany of CAS filed Critical Kunming Institute of Botany of CAS
Priority to CNB2007100657244A priority Critical patent/CN100529051C/en
Publication of CN101050424A publication Critical patent/CN101050424A/en
Application granted granted Critical
Publication of CN100529051C publication Critical patent/CN100529051C/en
Expired - Fee Related legal-status Critical Current
Anticipated expiration legal-status Critical

Links

Landscapes

  • Measuring Or Testing Involving Enzymes Or Micro-Organisms (AREA)
  • Breeding Of Plants And Reproduction By Means Of Culturing (AREA)

Abstract

This invention provides a method for preparing endophytes, i.e., enriching endophytic microbes from plant materials. The method comprises: centrifuging plant tissue pulp at a low speed to remove non-pulverized plant cell clusters and part of cell nuclei, further removing impurities such as cell nuclei, organelles and pectin by using haloid salt and surfactant, centrifuging at a high speed, and collecting the precipitate to obtain endophyte samples. It is proven that the enrichment effect of endophytes is obvious as detected by 16S rRNA gene technology of the prokaryotic microbes.

Description

The preparation method of endophyte of plant
Affiliated field:
The present invention relates to a kind of method of microorganism of from vegetable material, giving birth in the enrichment, just relate to a kind of preparation method of endophyte of plant.
Background technology:
No matter plant individual is a seed or a towering tree, all is a kind of ecotope of relative complex, and the microorganism that kind is different with abundance perches wherein; For living in plant tissue inside alive plant is not produced the microorganism of direct negative impact, be collectively referred to as endophyte of plant.Endophyte of plant is prevalent in plant materials and of a great variety, be gregarious in some privileged site of plant such as root nodule and the crown-gall nodule except that the small part endophyte is concentrated, most endophyte of plant disperse in plant materials usually and occupy, people to these endophytes perch the position and the kind diversity is known little about it.Moreover, most of environmental microorganism comprises that numerous endophyte of plant is difficult to artificial culture and survives, thereby can not carry out isolation identification and product chemical research by pure culture.In order to use the grand Study on Genome strategy of endophyte to excavate the genetic resources of endophyte of plant and to develop the potential that its compound produces, first step is from the vegetable material enriching plant endophyte and the interference of removing a large amount of plant genetic materials.Relevant report only has the method for enrichment soil microorganisms, its principle is to remove soil impurity by density gradient centrifugation, the inventor once adopted the method for this kind principle but can not effectively be enriched to endophyte from plant tissue, this is because there is the essence difference in the impurity that will remove, and the former is a soil particle and the latter is the plant genetic material.In order to reach from the purpose of vegetable material enrichment endophyte, the present inventor once reported usefulness cellulase and the macerozyme method (Journal of Applied Microbiology 100:830-837) from plant leaf and seed enrichment endophyte in 2006.Follow-up study finds that there is shortcoming in this method, and promptly enzyme action time is longer, may cause enriched sample endophyte abundance deviation because of growing of certain micro-organisms.
Summary of the invention:
The objective of the invention is to overcome the limitation of above-mentioned prior art, a kind of new endophyte of plant preparation method is provided.
In order to realize above-mentioned purpose of the present invention, the invention provides following technical scheme:
The preparation method of endophyte of plant, get vegetable material through high-speed tissue mashing machine's homogenate, low-speed centrifugal 200g * 5min gets supernatant liquor adding halogen sodium-chlor or lithium chloride to final concentration 0.1%~3.0%, is unit with the weight/volume, add tensio-active agent sodium laurylsulfonate or Triton X-100 again to final concentration 0.01~2.0%, with the weight/volume is unit, and mixing left standstill 1-2 hour, get supernatant liquor 5000g centrifugal 10 minutes, and obtained being precipitated as endophyte of plant.
The employed halogen of aforesaid method is preferably used the monovalent cation halogen, or the divalent cation halogen.
The employed tensio-active agent of aforesaid method is preferably with ionogenic surfactant or nonionic surface active agent.
Method of the present invention is based on a certain amount of vegetable material and sterilized water is handled with high-speed tissue mashing machine, homogenate is through the low-speed centrifugal after separating, remove plant origin impurity with certain density halogen and tensio-active agent and comprise nucleus, organoid and colloid etc., get supernatant liquor after the natural subsidence and just can obtain the abundant and very few enriched sample of plant genetic interfering substance of endophyte through the high speed centrifugation collecting precipitation.
Embodiment:
Below in conjunction with the furthermore bright essentiality content of the present invention of embodiments of the invention, but do not limit the present invention with this.
Embodiment 1:
Get trewianudiflora stem skin 40 grams, clean, add 300 ml sterile waters, with the 18000rpm of high-speed tissue mashing machine homogenate with tap water and distilled water; Filter tissue and the fiber of removing not fragmentation with sterile gauze, (200g * 5min) precipitation is removed in separation to filtrate with low-speed centrifugal; Add in the supernatant liquor sodium-chlor to final concentration 1.0% (w/v) and sodium laurylsulfonate to final concentration 0.05% (w/v), put upside down mixing and left standstill 1 hour, have a large amount of flockss and produce this moment, not the disturbance precipitation; The careful new sterilization centrifuge tube of supernatant liquor to of drawing, centrifugal 10 minutes of 5000g, the precipitation that obtains is the endophyte enriched sample.
Embodiment 2:
Get fresh blade 20 grams of Yunnan Caulis Mayteni, clean, add 400 ml sterile waters, with the 15000rpm of high-speed tissue mashing machine homogenate with tap water and distilled water; Filter to remove broken tissue and fiber with sterile gauze, filtrate is with the low-speed centrifugal (precipitation separation of 200g * 5min); Add in the supernatant liquor lithium chloride to final concentration 0.6% (w/v) and Triton X-100 to final concentration 0.15% (w/v), put upside down mixing and left standstill 2 hours, have a large amount of flockss and produce this moment, not the disturbance precipitation; The careful new sterilization centrifuge tube of supernatant liquor to of drawing, centrifugal 10 minutes of 5000g, the precipitation that obtains is the endophyte enriched sample.
Embodiment 3:
Get embodiment 1 or 2 resulting endophyte enriched sample, carry out the detection of endophyte concentration effect.Utilization does not rely on the 16S rRNA gene engineering of cultivation, extracts the DNA of endophyte enriched sample, with the DNA of 2 gram blades or stem skin in contrast, sets up 16S rDNA library; At least 100 clones of picking Pvu II enzyme of carrying out 16S rDNA amplified fragments is cut at random, can not may be derived from prokaryotic micro-organisms by the clone that Pvu II enzyme is cut; This part clone is carried out RFLP somatotype and dna sequencing, infer that according to 16S rDNA sequence this sequence derives from the prokaryotic cell prokaryocyte that plant chloroplast still is an endophyte.Compared with the control, in the enriched sample, the 16S rDNA clone's in prokaryotic micro-organisms source ratio and sequence polymorphism obviously increase (seeing Table 1), illustrate that the inventive method can access rich and varied endophyte of plant, and the plant genetic material disturbs obviously minimizing, thereby has reached from the purpose of vegetable material enrichment endophyte.
The detected result of table 1 endophyte of plant concentration effect of the present invention
Figure C20071006572400061
*Clone's molecular system type is represented the prokaryotic cell prokaryocyte source with pro;
Figure C20071006572400062
Prokaryotic cell prokaryocyte 16S rDNA clone accounts for total detection clone's percentage ratio.

Claims (1)

1, the preparation method of endophyte of plant, it is characterized in that vegetable material is through high-speed tissue mashing machine's homogenate, low-speed centrifugal 200g * 5min gets supernatant liquor adding halogen sodium-chlor or lithium chloride to final concentration 0.1%~3.0%, is unit with the weight/volume, add tensio-active agent sodium laurylsulfonate or Triton X-100 again to final concentration 0.01~2.0%, with the weight/volume is unit, and mixing left standstill 1-2 hour, get supernatant liquor 5000g centrifugal 10 minutes, and obtained being precipitated as endophyte of plant.
CNB2007100657244A 2007-03-19 2007-03-19 Method for preparing endophyte of plant Expired - Fee Related CN100529051C (en)

Priority Applications (1)

Application Number Priority Date Filing Date Title
CNB2007100657244A CN100529051C (en) 2007-03-19 2007-03-19 Method for preparing endophyte of plant

Applications Claiming Priority (1)

Application Number Priority Date Filing Date Title
CNB2007100657244A CN100529051C (en) 2007-03-19 2007-03-19 Method for preparing endophyte of plant

Publications (2)

Publication Number Publication Date
CN101050424A CN101050424A (en) 2007-10-10
CN100529051C true CN100529051C (en) 2009-08-19

Family

ID=38782024

Family Applications (1)

Application Number Title Priority Date Filing Date
CNB2007100657244A Expired - Fee Related CN100529051C (en) 2007-03-19 2007-03-19 Method for preparing endophyte of plant

Country Status (1)

Country Link
CN (1) CN100529051C (en)

Families Citing this family (6)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN101434906B (en) * 2008-12-19 2010-09-15 湖南大学 Separation process for plant endophyte
CN102191190A (en) * 2010-03-17 2011-09-21 北京龙裔生物科技有限公司 Potato with rich SOD complex enzyme and planting method thereof
CN101955903B (en) * 2010-09-28 2012-06-27 广州市永雄有机肥有限公司 Bacillus licheniformis bacterial strain and application thereof
CN103937719B (en) * 2014-04-22 2016-01-27 中国科学院新疆生态与地理研究所 A kind of method being separated euhalophyte endogenetic bacteria
CN112795513A (en) * 2021-02-03 2021-05-14 南京翠京元生物科技有限公司 Enrichment and separation method for endophyte
CN113913411A (en) * 2021-12-01 2022-01-11 北京林业大学 Composition for extracting fungal protoplast from plant and application thereof

Non-Patent Citations (4)

* Cited by examiner, † Cited by third party
Title
Enrichment for microbes living in association with plant tissues. J.-Y. Jiao, H.-X. Wang, Y. Zeng, Y.-M. Shen.Journal of Applied Microbiology,Vol.100 . 2006
Enrichment for microbes living in association with plant tissues. J.-Y. Jiao,H.-X.Wang,Y. Zeng,Y.-M. Shen.Journal of Applied Microbiology,Vol.100. 2006 *
植物内生细菌研究进展及其应用潜力. 韩继刚,宋未.自然科学进展,第14卷第4期. 2004
植物内生细菌研究进展及其应用潜力. 韩继刚,宋未.自然科学进展,第14卷第4期. 2004 *

Also Published As

Publication number Publication date
CN101050424A (en) 2007-10-10

Similar Documents

Publication Publication Date Title
CN111876351B (en) Bacillus belgii and application thereof in relieving apple continuous cropping obstacle
CN105670958B (en) One plant of low temperature biocontrol bacterial strain and its application
CN100529051C (en) Method for preparing endophyte of plant
CN106167776A (en) A kind of can bacillus cereus (Bacillus cereus) TH 35 of heavy metal cadmium and application thereof in activating soil
CN103421717B (en) A kind of Bacillus cercus and application thereof
CN110200018B (en) Optimal DSE inoculation amount for promoting plant rooting
CN102888354A (en) Lysinibacillusfusiformis and method for degrading microcystis aeruginosa by using lysinibacillusfusiformis
CN104371956B (en) There is bacillus and the purposes of blocking effect to cadmium
KR101563349B1 (en) Microorganism mixture of arbuscular mycorrhizal fungi and Massilia sp. RK4 promoting plant growth under salt stress condition and uses thereof
AU2018402480A1 (en) Endogenous bacillus megaterium BM18-2 with cadmium enrichment for promoting growth of hybrid pennisetum and application thereof
CN106801017A (en) The cordyceps militaris link bacterial strain screening of a kind of high yield thermophilic protease and cordycepin and method of mutagenesis
CN111471621B (en) Water area microbacterium MB338 and application thereof
CN103555584B (en) Acquisition and application of grease-producing monoraphidium LB50
CN103981101B (en) A kind of DSE bacterial strain and the application in sugarcane production thereof
CN104498372B (en) Fusarium oxysporum BM201, its compound pectinase produced and compound pectinase preparation method and application
CN107384804B (en) Gibberella NT-1 and application thereof
CN108841748A (en) Sinorhizobium nitrogen-fixing bacteria strain H6 and its application
CN103451116B (en) Pseudomonas fluorescens Y13, and preparation method and applications thereof
CN105176855B (en) One plant of Sphingomonas bacterium obtained through separation and its application in continuous cropping watermelon growing is promoted
CN101519684B (en) Method for screening pseudomonas syringae pv.tabaci antagonistic bacteria
CN113930358B (en) Bacterial strain capable of decomposing kelp
CN106591173A (en) Bacillus flexus HL-37 capable of activating soil heavy metal cadmium, and applications thereof
CN103540533B (en) Obtaining and application of oil-producing monoraphidium LB59
CN106416835B (en) Utilize the method for bacillus atrophy bacillus BA-7 prevention and treatment Cruciferae clubroot
CN113005041B (en) Diamond algae, culture method thereof and application thereof in super-salt oil production

Legal Events

Date Code Title Description
C06 Publication
PB01 Publication
C10 Entry into substantive examination
SE01 Entry into force of request for substantive examination
C14 Grant of patent or utility model
GR01 Patent grant
C17 Cessation of patent right
CF01 Termination of patent right due to non-payment of annual fee

Granted publication date: 20090819

Termination date: 20130319