CN105861332B - A kind of bacterial strain of the promotion with leaf pocket orchid plant strain growth and its application - Google Patents

A kind of bacterial strain of the promotion with leaf pocket orchid plant strain growth and its application Download PDF

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CN105861332B
CN105861332B CN201610389267.3A CN201610389267A CN105861332B CN 105861332 B CN105861332 B CN 105861332B CN 201610389267 A CN201610389267 A CN 201610389267A CN 105861332 B CN105861332 B CN 105861332B
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pocket orchid
growth
promotion
leaf pocket
cortinarius
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CN105861332A (en
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周主贵
王晓国
黄昌艳
何荆洲
李秀玲
卢家仕
李冬萍
邓杰玲
陈廷速
张自斌
卜朝阳
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Flower Research Institute Guangxi Academy Of Agricultural Sciences
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Flower Research Institute Guangxi Academy Of Agricultural Sciences
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    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
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    • C12R2001/00Microorganisms ; Processes using microorganisms
    • C12R2001/645Fungi ; Processes using fungi
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    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N1/00Microorganisms, e.g. protozoa; Compositions thereof; Processes of propagating, maintaining or preserving microorganisms or compositions thereof; Processes of preparing or isolating a composition containing a microorganism; Culture media therefor
    • C12N1/14Fungi; Culture media therefor
    • C12N1/145Fungal isolates

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Abstract

The invention belongs to plant growth-promoting bacteria technical fields, and in particular to be a kind of bacterial strain of the promotion with leaf pocket orchid plant strain growth and its application.A kind of bacterial strain of the promotion with leaf pocket orchid plant strain growth, taxology are named as Cortinarius b-2-2 (Cortinarius sp.), and Guangdong Province's Culture Collection is preserved on May 12nd, 2016, and deposit number is GDMCC No.60037.The bacterial strain of promotion of the invention with leaf pocket orchid plant strain growth is promoting with the application in leaf pocket orchid plant strain growth.Band leaf pocket orchid plant strain growth is promoted using method provided by the invention, it is easy to operate, low in cost.The present invention gives birth to important economic value for the artificial breeding with leaf pocket orchid.

Description

A kind of bacterial strain of the promotion with leaf pocket orchid plant strain growth and its application
Technical field
The invention belongs to plant growth-promoting bacteria technical fields, and in particular to be a kind of bacterium of the promotion with leaf pocket orchid plant strain growth Strain and its application.
Background technique
Paphiopedilum (Paphiopedilum) plant, flower-shape is peculiar, and pattern is gorgeous, be the favorite orchid of people it One, often pocket orchid is referred to as " slippers are blue ", " celestial being is carried out blue " to people.In recent ten years, due to wildness smuggling and habitat destruction etc., The quantity of Wild Paphiopedilum is sharply reduced, distributed area gradually atrophy, and many types have arrived the edge of extinction.
In order to alleviate the acquisition pressure to Wild plant, endangered species is protected, and meet people to cypripedium Demand, domestic and foreign scholars study the artificial propagation of pocket orchid plant in large quantities.Currently, sterile the broadcasting of part pocket orchid species class Kind and tissue culture technique have succeeded, but slow growth after aseptic seedling cultivation, and survival rate is low, restricts the artificial breeding of pocket orchid It educates.Under field conditions (factors), the Seedling Stage that mycorrhizal fungi can help plant to spend fragility grows up to plant, improves plant and improves nutrient Absorption efficiency and adverse circumstance resistance.But because cypripedium mycorrhizal fungi is separately cultured difficulty, still lack with more aobvious The growth-promoting bacterial strain of work.Therefore, screening and cultivate to have promotes the bacterial strain of pocket orchid plant strain growth to restore tool to the cultivation of pocket orchid and population It is significant.
The information disclosed in the background technology section is intended only to increase the understanding to general background of the invention, without answering When being considered as recognizing or imply that the information constitutes the prior art already known to those of ordinary skill in the art in any form.
Summary of the invention
The object of the present invention is to provide a kind of bacterial strain of the promotion with leaf pocket orchid plant strain growth and its applications.
Strain b- -2-2 provided by the invention be it is isolated from Paphiopedilum micranthum root, reflect through morphology and molecular biology It is set to the Cortinarius (Cortinarius sp.) of Basidiomycotina Agaricales, is preserved in Guangdong Province on May 12nd, 2016 Culture Collection (abbreviation GDMCC, address: 5 building, the building of compound the 59th of Xianlie Middle Road, Guangzhou City 100, the micro- life in Guangdong Province Object research institute, postcode 510075), deposit number is GDMCC No.60037.
The present invention also provides the strains A 6-2 to promote with the application in leaf pocket orchid plant strain growth.
Compared with prior art, the invention has the following beneficial technical effects:
1. strain b- -2-2 of the invention can promote seedling development with the co-cultivation of leaf pocket orchid plant, grows and can be carried out light The blade of cooperation cultivates seedling replanting to matrix, and seedling can survive and well-grown.
2. band leaf pocket orchid breeding efficiency and process are promoted using method provided by the invention, it is easy to operate, low in cost.This Invention gives birth to important economic value for the artificial breeding with leaf pocket orchid.
Preservation information explanation
Cortinarius b-2-2 (Cortinarius sp.), deposit number are GDMCC No.60037, the deposit date is On May 12nd, 2016, depositary institution are Guangdong Province's Culture Collection (GDMCC), and preservation address is Guangzhou martyr 5 building, the building of compound the 59th of Road 100.
Detailed description of the invention
Fig. 1 is the molten bacterium of Cortinarius b-2-2 (Cortinarius sp.) of the invention on PDA solid medium Fall form;
Fig. 2 is the hypha form of Cortinarius b-2-2 (Cortinarius sp.) of the invention;
Fig. 3 is that microbial inoculum prepared by Cortinarius b-2-2 (Cortinarius sp.) of the invention compares plant strain growth Figure;
Explanation in relation to appended drawing reference:
CK is the plant that microbial inoculum of the invention is not used;B-2-2 is using Cortinarius b-2-2 of the invention The plant of the microbial inoculum of (Cortinarius sp.) preparation.
Specific embodiment
Below with reference to specific embodiment, the present invention is described in further detail, it is described be explanation of the invention and It is not to limit.
Material and reagent as used in the following examples, are commercially available unless otherwise specified.Following implementations Experimental method used in example is conventional method unless otherwise specified.
Embodiment 1: the separation identification and culture of mycorrhizal fungi
1.1 separation and pure medium
Separating mycorrhizal fungi culture medium is potato dextrose medium (PDA), potato 200g, agar 6g, glucose To 1000ml, PH is natural for 15g moisturizing.According to conventional biology test method, isolation medium is configured, 121 DEG C of high pressures are damp and hot to go out Bacterium 20min is cooled to 45 DEG C or so to culture medium, streptomysin (100ug/ml) and penicillin (100ug/ml) is added, after shaking up Prepare plate.
The separation of 1.2 mycorrhizal fungis and purification process
Mycorrhizal fungi separates according to conventional organization partition method: taking the Lanzhou-Xinjiang fresh feeding root of band leaf pocket, is chosen at Leica microscope Lower observation selection has the root segment of hypha body, rinses well under flowing water, handles 8min, sterile water respectively with the rinsing of 75% alcohol It rinses 1-2 times, then sterilizes 8min, aseptic water washing 7-8 times with 10%NaClO.Pretreated root is cut into the small of 1-2mm The material handled well, is then placed on PDA plate, 24 DEG C of constant temperature incubation 3-5d, it is seen that the bacterium grown out of cortical cell by section Filament length enters in culture medium.Bacterial strain is separated and purified using mycelia tip picking method, then is connected in test tube and saves.
The Morphological Identification of 1.3 mycorrhizal fungis
Observe the colony characteristics of bacterial strain, including colony shape, size, color, the speed of growth and mycelia, sporophore and spore Form etc..Observation discovery is in PDA culture medium, and bacterium colony is at milky, and early stage mycelia is close to culture basal growth, and edge pole is not advised Then;Later period can produce a large amount of aerial hyphaes, and form carpet veneer shape subiculum, and bacterium colony is at milk yellow;The relatively slow about 5.5d of mycelia growth Left and right can cover with culture dish;Mycelia is without every Hyphal anastomosis degree is high, easily forms Hyphal anastomosis circle;Do not generate spore.
Method for identifying molecules: the collection of mycelia: strain inoculated to PDA liquid medium is shaken into bacterium 7-10 days (200rpm, 25 DEG C), mycelia is collected by filtration in filter paper, extracts for genome.Genome DNA extraction uses CTAB method.
The PCR amplification of ITS section: the amplification of rDNA ITS section uses universal primer ITS1 (5 ' TCCGTAGGTGAACCTGCGG3 '), ITS4 (5 ' TCCTCCGCTTATTGATATGC3 ').The group of PCR reaction system become 10 × Buffer 5ul, 10mmol/L NTP (Mg+) 1ul, each 1ul of 10u mol/L primer, (final concentration is in 80ng/L by template DNA 1ul Left and right), Taq enzyme 1U (0.25ul) is settled to 50ul with sterile pure water.PCR reaction uses BIARAD Engine type PCR instrument, follows Ring parameter are as follows: 95 DEG C of initial denaturation, 4min, be denaturalized 95 DEG C, 40s, anneal 56 DEG C, 40s, extend 72 DEG C, 45s;72 DEG C of filling-in, 8min.35 circulations are carried out altogether.
Product send to Beijing AudioCodes biotechnology Co., Ltd and (the use of instrument being ABI 3730XL) is sequenced.Institute It obtains sequence results and carries out comparison by Internet using PRIMER3 software, and be aided with artificial check and correction, determine the reliability of sequence.Obtain sequence It is listed in BLAST on NCBI.
Sequencing result is as shown in sequence 1 in sequence table.Sequencing result is compared online in GenBank, the bacterial strain with The similitude of Cortinarius (Cortinarius sp.) is higher, determines that the bacterial strain being separated to is Tulasnella fungi, is named For strain b- -2-2.
Embodiment 2: the preparation and application of microbial inoculum
The preparation of 2.1 liquid bacterial agents and application
Using PDA liquid medium (potato 200g, glucose 15g moisturizing to 121 DEG C of high pressure moist heat sterilizations of 1000mL) 20min is cooled to room temperature to culture medium.Bacterium 20d or so is shaken with 160-220rpm in shaking table after inoculating strain A6-2, dilutes bacterium solution 200-300 times, root dipping or pouring root, about 60d pouring root 1 time are carried out to the tissue-cultured seedling transplanted in the recent period.Tissue-cultured seedling bottle outlet requires to be root long At least in 2cm or more, 3 plant with blade can just be transplanted.
The preparation of 2.2 solid fungicides and application
By cultivation matrix (pine bark about 2m2Size: perlite 4:1) be dipped into it is wet in 121 DEG C of high pressures after complete water saturation Heat sterilization 20min, is cooled to room temperature to culture medium.In 30 DEG C of placement 25d or so after the microbial inoculum of inoculating strain A6-2 preparation, until Until observing after bark has milky, tissue-cultured seedling is transplanted after the matrix that will carry disease germs packing.
Transplanted seedling about 180d, random each selection after transplanting of microbial inoculum (control) is not applied to application microbial inoculum (b-2-2) and 30 plants of progress numbers of blade, most come into leaves, radical, longest root and fresh weight measure, the results are shown in Table 1.
The microbial inoculum of the Cortinarius b-2-2 of the invention of table 1 (Cortinarius sp.) preparation is to band leaf pocket orchid plant biology The influence of amount
Note: different lowercases indicate 0.05 horizontal upper significant difference after data;Different capitalizations indicate that 0.01 is horizontal On significant difference.
As shown in Table 1, the band leaf of the microbial inoculum of Cortinarius b-2-2 of the invention (Cortinarius sp.) preparation is applied Pocket orchid plant root long degree dramatically increases, and fresh weight increase is also extremely significant.
In conclusion microbial inoculum prepared by Cortinarius b-2-2 (Cortinarius sp.) of the invention can dramatically increase The leaf growth of plant promotes the elongation of root, increases the accumulation of biomass.
The aforementioned description to specific exemplary embodiment of the invention is in order to illustrate and illustration purpose.These descriptions It is not wishing to limit the invention to disclosed precise forms, and it will be apparent that according to the above instruction, can much be changed And variation.The purpose of selecting and describing the exemplary embodiment is that explaining specific principle of the invention and its actually answering With so that those skilled in the art can be realized and utilize a variety of different exemplary implementation schemes of the invention and Various chooses and changes.The scope of the present invention is intended to be limited by claims and its equivalents.

Claims (2)

1. a kind of bacterial strain of the promotion with leaf pocket orchid plant strain growth, taxology are named as Cortinarius (Cortinarius sp.) B-2-2, Guangdong Province's Culture Collection is preserved on May 12nd, 2016, and deposit number is GDMCC No.60037.
2. bacterial strain of the promotion with leaf pocket orchid plant strain growth described in claim 1 is promoting with answering in leaf pocket orchid plant strain growth With.
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Families Citing this family (5)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN107746811B (en) * 2017-10-30 2020-04-03 广西壮族自治区农业科学院花卉研究所 Strain for promoting growth of paphiopedilum hirsutissimum plants and application thereof
CN110760448B (en) * 2019-11-08 2022-03-22 广西壮族自治区农业科学院 Strain for promoting growth of paphiopedilum hirsutissimum plant and application thereof
CN112592838B (en) * 2020-12-31 2022-11-29 广西壮族自治区林业科学研究院 Orchid mycorrhizal fungus PF07 and application thereof
CN112646734B (en) * 2020-12-31 2022-11-29 广西壮族自治区林业科学研究院 Orchid mycorrhizal fungus PF06 and application thereof
CN112795489B (en) * 2020-12-31 2022-11-29 广西壮族自治区林业科学研究院 Orchid mycorrhizal fungus PF02 and application thereof

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CN103087927A (en) * 2013-01-21 2013-05-08 北京林业大学 Fungus for promoting symbiotic germination of paphiopedilum hirsutissimum seed and application thereof
CN104920462A (en) * 2015-06-09 2015-09-23 柳州市天姿园艺有限公司 Composition for controlling leaf spot disease of paphiopedilum

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CN103087927A (en) * 2013-01-21 2013-05-08 北京林业大学 Fungus for promoting symbiotic germination of paphiopedilum hirsutissimum seed and application thereof
CN104920462A (en) * 2015-06-09 2015-09-23 柳州市天姿园艺有限公司 Composition for controlling leaf spot disease of paphiopedilum

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