CN101205525A - Recombinant saccharomyces cerevisiae for producing ethanol by using xylose and glucose - Google Patents
Recombinant saccharomyces cerevisiae for producing ethanol by using xylose and glucose Download PDFInfo
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Abstract
The invention belongs to the bioengineering technical field and discloses a Saccharomyces cerevisiae YPH499-3 which has been collected in China General Microbiological Culture Collection Center of China Committee for Culture Collection of Microorganisms with a collection number of CGMCC No.2255. The Saccharomyces cerevisiae of the invention can well utilize xylose and also can simultaneously transport the xylose and glucose to produce ethanol, and utilization rate reaches over 80 percents.
Description
Technical field
The invention belongs to technical field of bioengineering, be specifically related to a kind of wood sugar that can utilize and also can utilize wood sugar and glucose production alcoholic acid recombinant Saccharomyces cerevisiae (Saccharomyces cerevisiae) YPH499-3 simultaneously.
Background technology
Lignocellulose is the abundantest in the world biomass resource, and amount is maximum, valency is the most honest and the cleanest, and annual ultimate production accounts for 50% of all biomass resources, and this type of material of great majority is not well utilized at present.Utilize lignocellulose to be main renewable biomass resource, the production renewable energy source has important economy and society meaning.With biomass is the industrial alcohol that raw material is produced, and as a kind of renewable energy source of cleaning, is the inexorable trend that substitutes fossil oils such as oil.Traditional bio-ethanol production is mainly based on the grain fermentation, and world food phenomenon in short supply has seriously limited raw material sources, and raw materials cost is high, and the new raw material route is the key that reduces the bio-ethanol production cost cheaply.In traditional bio-ethanol is produced, be easy to by microbial fermentation generation ethanol based on the hexose of glucose, yet the wood sugar that accounts for total reducing sugar amount about 40% but is not easy to by its utilization.Ethanol is produced in the wood-sugar fermentation that makes full use of in the lignocellulose production ethanol raw material, can make alcoholic acid output increase by 25% on the original basis.Effective utilization of wood sugar is the important content that improves the ethanol economic target, is the key factor that biomass resource success industrialization transforms.
Yeast saccharomyces cerevisiae (S.cerevisiae) is an eukaryotic microorganisms, and cell wall thickness, sterol content height are higher to the tolerance of the ethanol and the lignocellulose hydrolyzate toxic factor; Can be under low pH, strictly anaerobic condition quick fermentation glucose production ethanol, by product is few; Be difficult for by bacterium and virus pollution, and the related industries technology maturation, be the research emphasis and the preferred object microorganism of ethanol fermentation always.But lack the ability of effectively utilizing wood sugar.With the lignocellulose is raw material production ethanol, and one of its key is exactly to produce the alcoholic acid microorganism can effectively utilize various sugar as carbon source.Abroad, as far back as the eighties initial stage in last century, its High-efficient Production alcoholic acid research has just been taken in many in the world laboratories.But natural S. cervisiae is the metabolism wood sugar very slowly, but effective xylose-fermenting.Because the wood-sugar fermentation performance of natural microbial is difficult to reach industrial requirement, so people utilize traditional bacterial screening method to cultivate the required bacterial classification of seed selection through a large amount of microorganism culturing, enzyme activity determination and strain domestications usually, because big, the consuming time length of workload, efficient are low, turned in recent years and utilized the metabolic engineering principle, by molecular genetic transform the associated metabolic approach obtain can under anaerobic efficient metabolism glucose fermentation, the engineering bacteria of wood sugar and other various pentoses.But research major part does not in the past obtain very good target phenotype.We think the transformation of these single-genes or several genes, certain genetically deficient or amplification, just change the local element of cell, or redesigned the equilibrium system of having regulated the cellular network meta-bolites, do not solved the challenge in the xylose metabolism approach.
Gene expression regulation is also to become biology to use the means focus at present.The overall situation is transcribed mechanism regulating engineering (globetranscriptional mechanism engineering, gTME) be to use molecular biology method, as methods such as fallibility PCR, DNA reorganization, set up the sudden change storehouse of general transcription factor, at purpose product or target phenotype, by directed screening, obtain purpose metabolism stream and strengthen or particular phenotype enhanced bacterial classification, be a kind of method that obtains the target phenotype by people's design.
Yeast saccharomyces cerevisiae has the complete approach of xylose metabolism, but but effective xylose fermentation ethanol.We address these problems the change that the simulation microorganism adapts to external environment, orthogenesis or change a plurality of genes involved groups simultaneously on the genome aspect of yeast xylose metabolism approach, make cell on integral level, adapt to the metabolism or the utilization of wood sugar, thereby we utilize the gTME technology whole transcriptional control process to be changed change or improve by gene engineering method transformation overall situation transcriptional regulator genomicly to transcribe and express.Thereby obtained efficiently to utilize wood sugar also can transport the yeast saccharomyces cerevisiae of wood sugar and glucose producing and ethanol simultaneously.
Utilize global regulation's technology engineered to the S. cervisiae mechanism of transcribing, screening obtains the bacterial strain that utilizes wood sugar high.And cooperate aimed strain to make a concrete analysis of, further investigation utilizes the metabolic regulation network and the mechanism of wood sugar, find out the influence of global regulation to the yeast saccharomyces cerevisiae xylose metabolism, wish to optimize yeast saccharomyces cerevisiae xylose metabolism network by the means of global regulation, realizing the xylose utilization of maximum efficiency, and efficiently utilize the wood sugar producing and ethanol to lay the foundation for yeast saccharomyces cerevisiae.Molecular breeding and the metabolic engineering strong for universality provide the solid engineering theory basis that is rich in new meaning, thereby make the cellular elements genetic evolution, realization by numerous and slowly to the letter and fast fundamental shifts, fundamentally reduce the raw materials cost of bio-ethanol, this will bring great innovation to the development of genetically engineered and metabolic engineering technical know-how, realize that the industrial application of recombinant bacterial strain also will have immeasurable huge pushing effect and more wide application prospect.
Summary of the invention
The objective of the invention is to provide a kind of for fear of above-mentioned weak point utilizes wood sugar and can transport wood sugar and glucose production alcoholic acid recombinant Saccharomyces cerevisiae (Saccharomyces cerevisiae) YPH499-3 simultaneously.
Purpose of the present invention reaches by following measures:
A kind of recombinant Saccharomyces cerevisiae of seed selection of inventor laboratory and preservation (Saccharomyces cerevisiae) YPH499-3, this yeast saccharomyces cerevisiae is preserved in China Committee for Culture Collection of Microorganisms common micro-organisms center (being called for short CGMCC) at present, the numbering of registering on the books is CGMCC No.2255, and preservation date is: on November 13rd, 2007.
The selection of this yeast saccharomyces cerevisiae CGMCC No.2255 is characterized in that utilizing the overall situation to transcribe machine-processed engineering (globalTransciption Machinery Engineering gTME) method, the screening of uridylic defective type wood sugar substratum.
1) starting strain
Starting strain is that (Saccharomyces cerevisiae YPH499 is available from U.S. Stratagene company, ura3-52 lys2-801 for yeast saccharomyces cerevisiae YPH499
AmberAde2-101
OchreTrp1-Δ 63 his3-Δs 200 leu2-Δs 1) be leucine, Histidine, uridylic defective type.
2) substratum
Minimum medium (YPD): yeast powder 10g, peptone 20g, glucose 20g, deionized water is settled to 1L.
Screening culture medium: do not contain amino acid yeast nitrogen (YNB) 6.7g, indispensable amino acid mixture (lacking uridylic) 1.3g,
Wood sugar 20g, agar powder 20g, deionized water is settled to 1L.
Seed culture medium: same minimum medium.
Fermention medium A (containing 5% wood sugar): yeast powder 10g, peptone 20g, wood sugar 50g, deionized water is settled to 1L.
Fermention medium B (containing 10% wood sugar): yeast powder 10g, peptone 20g, wood sugar 100g, deionized water is settled to 1L.
Fermention medium C (containing 15% wood sugar): yeast powder 10g, peptone 20g, wood sugar 150g, deionized water is settled to 1L.
Fermention medium D (containing 5% glucose): yeast powder 10g, peptone 20g, glucose 50g, deionized water is settled to 1L.
Fermention medium E (containing 10% glucose): yeast powder 10g, peptone 20g, glucose 100g, deionized water is settled to 1L.
Fermention medium F (containing 15% glucose): yeast powder 10g, peptone 20g, glucose 150g, deionized water is settled to 1L.
Fermention medium G (containing 5% mixing sugar): yeast powder 10g, peptone 20g, wood sugar 25g, glucose 25g, deionized water is settled to 1L.
Fermention medium H (containing 10% mixing sugar): yeast powder 10g, peptone 20g, wood sugar 50g, glucose 50g, deionized water is settled to 1L.
Fermention medium I (containing 15% mixing sugar): yeast powder 10g, peptone 20g, wood sugar 75g, glucose 75g, deionized water is settled to 1L.
Add 2% agar during preparation solid plate substratum.
3) mutagenesis of mutant strain and screening
Meet a ring yeast saccharomyces cerevisiae YPH499 and go into minimum medium, 30 ℃, 200r/min are cultivated 14h, centrifugal collection thalline, utilize pastoris genomic dna to extract test kit (TIANGEN company) extraction and obtain the YPH499 genome, to obtain the YPH499 genome is template, primer SPT15_Sense:TCGAGTGCTAGCAAAATGGCCGATGAGGAACGTTTAAAGG (SEQ ID No.2) and SPT15_Anti:CTAGCGGTCGACTCACATTTTTCTAAATTCACTTAGCACA (SEQ ID No.3), the clone obtains spt15 gene (SEQ ID No.1); Spt15 gene with acquisition is that template is carried out fallibility PCR[GenemorphII RandomMutagenesis kit (purchasing the Stratagene company in the U.S.)], gained fallibility PCR product is directly connected on PYX212 (the amicillin resistance band uridylic selection markers) expression vector, and the Lithium Acetate method is transformed into yeast saccharomyces cerevisiae YPH499 and expresses on screening culture medium.
By the particular screen culture medium condition, obtain and with the wood sugar to be the recombinant Saccharomyces cerevisiae YPH499-3CGMCC No.2255 that grows on the screening culture medium of sole carbon source, by the visible yeast saccharomyces cerevisiae YPH499-3 of microscopy CGMCC No.2255 (see figure 1).Yeast saccharomyces cerevisiae YPH499-3 CGMCC No.2255 is carried out shake flask fermentation in above-mentioned different fermentations substratum, the utilization ratio that records sugar in fermentation in the time of four days is: 94.0% (5% wood sugar), 90.0% (10% wood sugar), 82.0% (15% wood sugar), 98.9% (5% glucose), 97.1% (10% glucose), 95.9% (15% glucose), 91.7% (wood sugar in 5% mixing sugar), 85.9% (glucose in 5% mixing sugar), 80.8% (wood sugar in 15% mixing sugar), 90.3% (wood sugar in 10% mixing sugar), 92.0% (glucose in 10% mixing sugar), 92.1% (glucose in 15% mixing sugar), its wood sugar and glucose utilization rate all reach more than 80% and (the results are shown in Figure 2-4).Xylitol output is (fermented 109 hours: the Xylitol content of 10% wood sugar, 15% wood sugar is respectively: 2.81g/L, 2.45g/L.) seldom.
Recombinant Saccharomyces cerevisiae YPH499-3 CGMCC No.2255 has following character:
(1) colonial morphology feature: unicellular, be oval, circle or avette.The about 1-5 of size * 5-30 micron, atrichia can not move about.Bacterium colony smooth surface, moistening, thickness are provoked easily on solid medium, and the bacterium colony quality is even, and the color of pros and cons and edge, central part is homogeneous very all, and bacterium colony mostly is oyster white, and minority is red.Liquid culture is evenly grown.
(2) physiology and biochemical characteristic: have typical eucaryotic cell structures, cell walls, cytolemma, nucleus, tenuigenin, vacuole, plastosome etc. are arranged, what have also has a microbody.Amphimicrobian, vegetative propagation is based on budding.Energy glucose fermentation, wood sugar.
(3) nutritional character: heterotrophism.
Analytical procedure:
The centrifuge tube that will contain the 1.5ml fermented liquid places supercentrifuge, centrifugal 5min under 12000rpm, and it is standby to get supernatant.
Wood sugar, Xylitol, glucose concn high-performance liquid chromatogram determination.DIONEX (Ultimate3000) high performance liquid chromatograph, detector Shodex RI-101, the ChromeleonVersion6.80 workstation, chromatographic column is Kromasil5-NH2 post (Hanbon Sci. ﹠ Tech. Co., Ltd.) chromatographic condition: 30 ℃ of column temperatures, moving phase is acetonitrile: water=80: 20 (V/V), flow velocity are 1.0mL/min.
Ethanol detects: blood ethanol test kit (Changchun remittance power Bioisystech Co., Ltd), adopt two point velocity methods.
Cell concentration is measured with OD600,1OD600=0.367g dry mycelium/L (wood sugar), 0.410g dry mycelium/L (glucose), 0.355g dry mycelium/L (mixing sugar).
Beneficial effect of the present invention:
Recombinant Saccharomyces cerevisiae YPH499-3 CGMCC No.2255 optimum growth temp is 30 ℃, can well utilize wood sugar, and transport wood sugar and glucose simultaneously.Utilize wood sugar and glucose simultaneously, utilization ratio is all up to more than 80%.Be merely that sole carbon source fermenting alcohol productive rate is 5% with the wood sugar, wood sugar and glucose during with mixed fermentation in 1: 1 alcohol yied be 10%.
With other bacterial strains carry out effect relatively:
Yeast saccharomyces cerevisiae YPH499 is not long on pure wood sugar substratum, utilizes glucose when glucose and wood sugar exist simultaneously; Recombinant Saccharomyces cerevisiae YPH499-3 CGMCC No.2255 pure wood sugar, glucose and wood sugar the two etc. in the mixing sugar of quality sugared utilization ratio all reach more than 80%.
Description of drawings:
Fig. 1 is recombinant Saccharomyces cerevisiae YPH499-3 CGMCC No.2255 microscopy result.
Fig. 2 is the growth curve chart of recombinant Saccharomyces cerevisiae YPH499-3 CGMCC No.2255 on fermention medium.
Fig. 3 is the graphic representation that utilizes of wood sugar, glucose.
Fig. 4 is the graphic representation that utilizes of mixing sugar.
The explanation of preservation information:
A kind of recombinant Saccharomyces cerevisiae (Saccharomyces cerevisiae) YPH499-3, this yeast saccharomyces cerevisiae is preserved in China Committee for Culture Collection of Microorganisms common micro-organisms center (being called for short CGMCC) at present, the address is the Datun Road, Chaoyang District, Beijing City, Institute of Microorganism, Academia Sinica.Classification called after Saccharomyces Cerevisiae in S accharomyces cerevisiae, the numbering of registering on the books is CGMCC No.2255, preservation date is: on November 13rd, 2007.
Embodiment:
The present invention is further elaborated by the following examples.
Starting strain:
Starting strain is yeast saccharomyces cerevisiae YPH499 (available from a U.S. Stratagene company), is leucine, Histidine, uridylic defective type.
Substratum:
Minimum medium (YPD): yeast powder 10g, peptone 20g, glucose 20g, deionized water is settled to 1L.
Screening culture medium: do not contain amino acid yeast nitrogen (YNB) 6.7g, indispensable amino acid mixture (lacking uridylic) 1.3g,
Wood sugar 20g, agar powder 20g, deionized water is settled to 1L.
Add 2% agar during preparation solid plate substratum
The mutagenesis of mutant strain and screening:
Meet a ring yeast saccharomyces cerevisiae YPH499 from fresh inclined-plane and go into minimum medium, 30 ℃, 200r/min are cultivated 14h, centrifugal collection thalline, utilize pastoris genomic dna to extract test kit (TIANGEN) extraction and obtain the YPH499 genome, to obtain the YPH499 genome is template, primer SPT15_Sense:TCGAGTGCTAGCAAAATGGCCGATGAGGAACGTTTAAAGG (SEQ IDNo.2) and SPT15_Anti:CTAGCGGTCGACTCACATTTTTCTAAATTCACTTAGCACA (SEQ ID No.3), the clone obtains spt15 gene (SEQ ID No.1); Spt15 gene with acquisition is that template is carried out fallibility PCR[GenemorphIIRandom Mutagenesis kit (purchasing the Stratagene company in the U.S.)], gained fallibility PCR product is directly connected on PYX212 (the amicillin resistance band uridylic selection markers) expression vector, the Lithium Acetate method is transformed into yeast saccharomyces cerevisiae YPH499 and expresses on screening culture medium, obtains recombinant Saccharomyces cerevisiae bacterial strain YPH499-3 CGMCC No.2255.
Embodiment 2
Seed culture medium: yeast powder 10g, peptone 20g, glucose 20g, deionized water is settled to 1L.
Fermention medium: yeast powder 10g, peptone 20g, wood sugar 50g, deionized water is settled to 1L.
Meet the yeast saccharomyces cerevisiae YPH499-3 that a ring embodiment 1 obtains from fresh inclined-plane, CGMCC No.2255 inserts and is equipped with in the 50ml Erlenmeyer flask of seed culture medium, at 30 ℃, after cultivating 24h in the shaking table of 200rpm (Taicang experimental installation factory), be equipped with in the Erlenmeyer flask of fermention medium with 1% inoculum size (v/v) access, at 30 ℃, cultivate in the shaking table of 200rpm, fermentation 72h, the utilization ratio of gained wood sugar is 94%, alcohol yied is 5%.
Embodiment 3
Seed culture medium: yeast powder 10g, peptone 20g, glucose 20g, deionized water is settled to 1L.
Fermention medium: yeast powder 10g, peptone 20g, wood sugar 25g, glucose 25g, deionized water is settled to 1L.
Meet the yeast saccharomyces cerevisiae YPH499-3 that a ring is obtained by embodiment 1 from fresh inclined-plane, CGMCC No.2255 inserts and is equipped with in the Erlenmeyer flask of seed culture medium, at 30 ℃, behind the cultivation 24h, be equipped with in the Erlenmeyer flask of fermention medium in the shaking table of 200rpm (Taicang experimental installation factory) with 1% inoculum size (v/v) access, at 30 ℃, cultivate in the shaking table of 200rpm, fermentation 72h, the utilization ratio of gained wood sugar is 91%, the utilization ratio of glucose is 85%, and alcohol yied is 10%.
Claims (2)
1. recombinant Saccharomyces cerevisiae, its classification called after yeast saccharomyces cerevisiae (Saccharomyces cerevisiae) YPH499-3 has been preserved in China Committee for Culture Collection of Microorganisms common micro-organisms center, and its deposit number is: CGMCC No.2255.
2. the described recombinant Saccharomyces cerevisiae of claim 1 is utilizing wood sugar or is utilizing wood sugar simultaneously and glucose fermentation is produced application in the ethanol.
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