Long-chain biatomic acid production bacterial strain and its preparation method and application
Technical field
The present invention relates to a kind of strain and its preparation method and application, specifically a kind of long-chain biatomic acid production bacterial strain and
Its preparation method and application.
Background technology
Long-chain biatomic acid is important industrial chemicals, has extremely extensive purposes, being capable of synthetic perfume, extraordinary nylon, height
A series of chemicals of high added values such as level lubricating oil.Long-chain biatomic acid can be applicable to military domain, aerospace vehicle coating,
Pipeline, the face coat of automobile and oil pipe etc.;In civil area, automobile, daily use chemicals spices, engineering plastics, nylon row can be applied to
More than the ten individual high and new technology industry such as industry, can develop more downstream industries, form emerging industrial chain.
In the past, long-chain biatomic acid was produced using chemical synthesis, and its patented technology is possessed by foreign countries.Chemical synthesis is given birth to
Long-chain biatomic acid is produced, not only product category is single, and synthesis technique is complicated, cost is high, pollution is big.China is unique energy in the world
The country of a variety of long-chain biatomic acid large-scale industrial productions is enough realized using microbial fermentation technology.Before this, China's binary acid
The improvement of production strain is to educate method by the tradition such as different modes mutagenesis to realize.Traditional breeding way has very big random
Property, screening is complicated.Method by traditional breeding method has been difficult the further performance for improving bacterial strain.Current long-chain biatomic acid industry
Still there are many bottleneck problems during metaplasia production, such as substrate conversion efficiency has much room for improvement, energy consumption is very huge.
Metabolic engineering technology can targetedly carry out strain molecular modification on gene level, and it is more excellent to obtain performance
Good new strains.As shown in Figure 1 and Figure 2, binary acid metabolic pathway mainly includes omega oxidation approach and beta oxidation approach, wherein before
Person is binary acid route of synthesis, and the latter is related to binary acid degradation pathway.The purpose of metabolic engineering be by molecular modification means come
Omega oxidation activity is improved, and reduces beta oxidation activity.In the world, there are patent report in Henkel companies (later Cognis companies)
Road (US005254466A), optimize binary acid production bacterial strain with gene knockout mode, successively by 4 pox gene knockouts, reach
Beta oxidation is blocked completely, substrate conversion efficiency is risen to 100%.On this basis, the said firm further passes through metabolic engineering hand
Section coexpression CYP monooxygenases and reductase, to reach the purpose of enhancing omega oxidation, (the World Patent of output increased 30%
WO/91/06660)。
But batch fermentation experiment is carried out using the bacterial strain, its technique still can not be competing with other binary acid production processes at that time
Strive, and finally without progress large-scale production.Henkel companies carry out selection markers used in molecular modification to strain as urine
Pyrimidine auxotrophic.The shortcomings that Henkel companies patent of invention is:1st, starting strain is not the high yield used in industrialized production
Bacterial strain;2nd, the Candida used in Production of Long-chain Dicarboxylic Acids by Fermentation Methods is diploid, i.e., each cell has two sets of chromosomes, often
Individual gene has corresponding allele, and catalysis often walks the enzyme of internal biochemical reaction often by multiple gene codes.Therefore,
Strengthen or weaken the activity of some internal biochemical reaction, it is necessary to enter to the key gene for encoding the enzyme by metabolic engineering means
Row molecular modification just has remarkable result.Otherwise, effect also will not be notable after transformation.
The content of the invention
The present invention is exactly to solve the existing bacterial strain production inapparent technical problem of long-chain biatomic acid effect, there is provided a kind of
High long-chain biatomic acid production bacterial strain of production efficiency and its preparation method and application.
Therefore, the present invention provides a kind of long-chain biatomic acid production bacterial strain, its Classification And Nomenclature is candidiasis (Candida
Sp.) TDTC002, the bacterial strain were preserved in China Committee for Culture Collection of Microorganisms's commonly micro- life on March 18th, 2014
Thing center, abbreviation CGMCC, address are the institute 3 of Chaoyang District Beijing North Star West Road 1, Institute of Microorganism, Academia Sinica;Preservation
Numbering is:CGMCC No.8927.
Preferably, the ester acyl coenzyme A synthase gene in candidiasis has been knocked a copy.
Preferably, the ester acyl coenzyme A synzyme base being knocked be allele C andidaA00308 or
Candida01833, its base sequence is respectively as shown in the sequence 5 and sequence 6 of sequence table.The gene is in the strain gene group
Encode in multiple genes of the enzyme and produce the most key one for long-chain biatomic acid.
Present invention simultaneously provides a kind of preparation method of long-chain biatomic acid production bacterial strain, it comprises the following steps:(1) prepare
Primer ACS-FRTF and ACS-FRTR;(2) long-chain biatomic acid production bacterial strain competent cell, long-chain biatomic acid production bacterial strain are prepared
Candida (Candida sp.) DC12;(3) use the primer in step (1) to carry out expanding clonNAT resistant genes, utilize
The product of amplification knocks out to CandidaA00308 the or Candida01833 allele in strain, the allele
Base sequence respectively as shown in the sequence 5 and sequence 6 of sequence table;(4) expanded, purified by PCR, electricity turn, screening, identification,
Obtain long-chain biatomic acid production bacterial strain.
Preferably, long-chain biatomic acid produces the preparation method of bacterial strain in the present invention, screens the selection markers used in step
For clonNAT resistances.
Present invention simultaneously provides application of the long-chain biatomic acid production bacterial strain in long-chain biatomic acid is produced.
Preferably, after fermentation ends, zymotic fluid is heated to 70~80 DEG C;PH is adjusted to 9~9.5 again, thalline is removed and sinks
Form sediment, retain supernatant;To decolourize, temperature is maintained at 70~90 DEG C, obtains cleaner liquid, and pH2.5 is acidified to acid, and 70~90 DEG C are incubated,
Cooling, centrifugation or press filtration, washing, the precipitation after cleaning are dried in vacuo after taking out, and obtain long-chain biatomic acid.
Long-chain biatomic acid in the present invention refers to the unbranched dicarboxylic acid containing more than ten carbon atoms, is a kind of important essence
Refine work intermediate raw material, particularly SL-AH (DC12), DC14 (DC14), 16-dicarboxylic acid (DC16)
With DC18 (DC18).
The invention has the advantages that in order to break through the bottleneck of production strain genetic modification, the present invention is produced by parsing
The genomics and transcription group feature of bacterial strain, omega oxidation and beta oxidation metabolic pathway are analyzed, in genome global level really
Some related critical target points of binary acid metabolic have been found, then molecular modification is carried out to these sites by metabolic engineering means,
And verified by fermenting experiment, obtain the more excellent bacterial strain of performance.TDTC002 bacterial strain (the preserving numbers of the present invention:CGMCC
No.8927), it is improved compared to DC12 bacterial strains, conversion ratio, and what is more important is under conditions of fixed dissolved oxygen,
The required throughput and rotating speed all low compared with DC12 bacterial strains 25%~30% of TDTC002 bacterial strains, fermentation power consumption cost significantly reduce, and are
Large-scale production brings beneficial effect.
Brief description of the drawings
Fig. 1 be the present invention relates to long-chain biatomic acid synthesize related omega oxidation metabolic pathway;
Fig. 2 be the present invention relates to long-chain biatomic acid degrade related beta oxidation metabolic pathway;
Fig. 3 be the present invention relates to gene knockout flow chart;
Fig. 4 is the long-chain biatomic acid that HPLC analyzes DC12 fermenting and producings;
Fig. 5 is the long-chain biatomic acid that HPLC analyzes TDTC002 fermenting and producings.
The long-chain biatomic acid production bacterial strain of the present invention, its Classification And Nomenclature is candidiasis (Candida sp.)
TDTC002;Its preservation mechanism is China Committee for Culture Collection of Microorganisms's common micro-organisms center, abbreviation CGMCC, address
For Yard 1, BeiChen xi Road, Chaoyang District, Beijing City 3, Institute of Microorganism, Academia Sinica;Preservation date is March 18 in 2014
Day, preserving number numbering is:CGMCC No.8927.
Embodiment
In the present invention, sequence names are as follows in sequence table:Sequence 1:ACS-FRTF;Sequence 2:ACS-FRTR;Sequence 3:
ACS-U;Sequence 4:ACS-D;Sequence 5:CandidaA00308;Sequence 6:CandidaA01833.
The bacterium colony and thalli morphology observed in following examples are summarized as follows:
On solid medium flat board, bacterium colony cheese shape, surface is smooth, milky, and full projection, colony diameter is about 2mm.
Yeast sample is unicellular, and size is about 10x6 μm.In most cases, in the form of yeast sample is unicellular, while the pseudohypha bodily form is had
Into such as in the case where some growth phases or certain external condition stimulate, pseudohypha dramatically increases than regular meeting.
Culture medium set forth below has been used in following examples:
1st, YPD culture mediums, its formula are:1% yeast extract, 2% peptone, 2% glucose, if solid medium processed,
Add 2% agar powder.Above-mentioned percentage is quality percent by volume, i.e., the grams of the component needed for every 100 milliliters of culture mediums.If
Antibiotic is added, fluid nutrient medium adds to corresponding final concentration when in use.Solid medium is cooled to after autoclaving
During 50 degrees centigrade, antibiotic is added to corresponding final concentration, is fallen at once as in sterile culture dish after to be solidified after mixing
Put, be put in 4 degrees Celsius of refrigerators, used in two weeks.
2nd, the formula of seed culture medium:1~8g/L of yeast extract, 1~8g/L of corn steep liquor, sucrose 5~25g/L, KH2PO44~
12g/L, 0.5~4g/L of urea, 40~70g/L of weight wax, 121 DEG C sterilize 30 minutes.Wherein, sucrose and urea separately independent 110
DEG C sterilizing 20 minutes, mixing is remerged after sterilizing.
3rd, fermentation tank culture based formulas:1~8g/L of yeast extract, 1~8g/L of corn steep liquor, sucrose 5~30g/L, KH2PO44~
15g/L, urea 0.5~4g/L, KNO30.5~2.5g/L of 5~15g/L, NaCl, 121 DEG C sterilize 30 minutes.Wherein, sucrose
Separately individually sterilized with urea, 110 DEG C are sterilized 20 minutes, and mixing is remerged after sterilizing.75% glucose solution is prepared in addition,
105 DEG C sterilize 20 minutes, fermentation carry out initial stage stream plus.
Thalline culture set forth below and fermentation liquor treatment mode have been used in following examples:
1st, flat board culture:It is inverted in 30 DEG C of incubators, can be observed after the flat lining outs of YPD or coating within 2-3 days
Big and full milky bacterium colony is formed.
2nd, shaking table culture:Single bacterium is inoculated with flat board to drop down onto in fluid nutrient medium, or is come from fluid nutrient medium switching, 30 DEG C
Shaking table culture, rotating speed are maintained at 220 revs/min.
3rd, fermentation tank culture:Relatively more accurate in real time fermentation condition can be controlled, such as control of additive raw material, pH controls, dissolved oxygen control
With air agitation strength control etc..First stage, zymotic fluid pH controls are flowed 5~6.8 and add glucose solution, are bacterium
Body growth phase;Second stage, zymotic fluid pH is controlled 7.0~7.8, while (alkane, aliphatic acid or aliphatic acid spread out current adding substrate
Biology, such as methyl esters or ethyl ester), based on fermentation and acid, also growth part thalline;Phase III, acid is only produced, does not produce thalline,
According to fermentation situation continued current adding substrate (alkane, aliphatic acid or derivative of fatty acid, such as methyl esters or ethyl ester).Entirely fermented
Journey controls pH with 10M NaOH solutions auto-feeding, while dissolved oxygen is maintained at 20~40% by the adjustment of rotating speed.
4th, fermentation liquor treatment:After fermentation ends, zymotic fluid is heated to 70~80 DEG C, and maintain 60 minutes;Add 10M
PH is adjusted to 9~9.5 by NaOH, is removed bacterial sediment with tube centrifuge or press filtration, is retained supernatant;Proper amount of active carbon is added to take off
Color, temperature are maintained at 70~90 DEG C, and soaking time is 60 minutes;After removing activated carbon, cleaner liquid is obtained, with concentrated hydrochloric acid or dense sulphur
For sour continuously acidizing to pH2.5,70~90 DEG C are incubated 2 hours, are cooled to 30 DEG C, centrifugation or press filtration, clear water are washed one time, after cleaning
Precipitation is dried in vacuo after taking out, and obtains white long-chain biatomic acid.
Embodiment 1:Bacterial strain metabolic engineering
1) gene order-checking
Long-chain two is prepared using the genome extracts kit (Yeast DNAiso Kit) of precious bioengineering Co., Ltd
First acid production bacterial strain Candida genomic DNA, concrete operations are carried out according to kit specification.Genomic DNA is again by text
The steps such as storehouse structure, new-generation sequencing technology sequencing analysis and data assembling.By genome annotation and data analysis, obtain
Gene information of the bacterial strain in binary acid production correlation is produced, has excavated the bacterium in omega oxidation and beta oxidation metabolic pathway dependency basis
The coded sequence of cause.Two opening code-reading frame ester acyl coenzyme A synzyme of CandidaA00308 and Candida01833, base
Because length is 2157bp, sequence similarity is up to 96%, and upstream and downstream regional sequence is also highly similar, thus may determine that it is a pair
Allele.
2) transcript profile is sequenced
Long-chain biatomic acid production bacterium is prepared using the RNA extracts kits (RNeasy Mini Kit) of German Kai Jie companies
The total serum IgE of strain Candida, concrete operations are carried out according to kit specification.Obtained total serum IgE is again by library construction, transcription
Group sequencing and expression analysis.Aliphatic acid or long-chain biatomic acid need that after turning into ester acyl coenzyme A by activation β-oxygen could be entered
Change.And this single step reaction is to be catalyzed completion by ester acyl coenzyme A synzyme.By transcript profile data analysis, find
CandidaA00308 and Candida01833 this be respectively 2072.9 and 2001.5RPKM to equipotential gene transcription level.Here,
RPKM is a computational methods of gene expression amount, represents Reads Per Kb Per Million Reads.Its calculation formula
For
If RPKM (A) is the expression quantity of Gene A, then C is unique reads numbers compared to Gene A, and N arrives for unique comparison
Total reads numbers of reference gene, L are the base number of Gene A code area.RPKM methods can eliminate mrna length and sequencing amount difference pair
The influence of gene expression is calculated, the gene expression amount being calculated is used directly for icp gene differential expression.
Because beta oxidation is the related metabolic pathway of long-chain biatomic acid degraded, the purpose of strain transformation is to try to avoid binary
The generation of acid degradation.But another aspect beta oxidation is required for the metabolism of thalline normal physiological and energy supply.Therefore, wish
Prestige suppresses by the means of genetic engineering rather than blocks beta oxidation completely, and reaching neither influences thalline normal growth and long-chain
The synthesis of binary acid, the purpose for avoiding the long-chain biatomic acid of synthesis to be degraded again.CandidaA00308 and Candida01833 are
Diploid DC12 a pair of alleles, ester acyl coenzyme A synzyme is encoded, be responsible for activation aliphatic acid in binary acid degradation pathway
Or binary acid, ester acyl coenzyme A is generated, hence into beta oxidation metabolic pathway.Therefore, using metabolic engineering means, it is right to knock out this
The one of copy of allele, to reach the effect of suppressing binary acid degradation, so as to reach more efficient accumulation binary acid
Purpose.
3) gene knockout experiment flow is as shown in Figure 3.The design of design of primers principle, homology arm and detection primer all selects
The identical region in CandidaA00308 and Candida01833 comparison, knocked out so as to reach two allele
There is equal probability with detection.It is homology arm sequence at long primer ACS-FRTF and ACS-FRTR 5 ' ends, corresponding to gene
Knock out the upstream and downstream sequence in site.3 ' ends of the two long primers are respectively with knocking out module (deletion cassette)
Upstream and downstream pairing.The DNA fragmentation obtained after PCR amplifications, respectively with upstream and downstream homology arm, centre is resistance screening at two
Mark.
Electricity conversion is carried out after the DNA fragmentation of amplification is purified to import in somatic cells, the upstream and downstream homology arm of DNA fragmentation with
Double crossing over occurs for the target site on thalline chromosome, reaches the purpose of gene knockout.Because this double crossing over is small probability event,
Method for building up is needed to be screened.It is used here to resistant gene be Sat1, encode Knowles rhzomorph transacetylase.
Binary acid produces bacterial strain to Knowles rhzomorph (being called clonNAT or NTC) this medicaments insensitive, in the flat board of the rhzomorph containing Knowles
On can not grow, and thalline can decompose Knowles rhzomorph after expressing the enzyme, avoid lethal effect.Resistance screening mark is only whole
Closing to going to be expressed on chromosome, play a role so that thalline can grow on the culture medium flat plate containing resistance, and
Form bacterium colony.Simultaneously to resistant bacterium colony, purified and verified.
During checking, use to a pair of detection primers ACS-U and ACS-D, the upstream and downstream region with target site is matched somebody with somebody respectively
It is right.If there is no homologous recombination, by this pair of alleles be masterplate amplify come fragment be in length as
, a band can only be observed in agarose electrophoresis.If one of allele is because double cross-over event is by resistance base
Because fragment substituted for, then the fragment length obtained by amplification just changes, it is observed that two in agarose electrophoresis
Band.Verify that metabolic engineering obtains new strains in terms of binary acid production by the bacterial strain of checking, then by fermenting experiment
Whether advantage performance in is had.
4) PCR is expanded
Wherein, plasmid pSFS2, bibliography are Gene (2004) 341:The accession number of 119-127, GeneBank database
For:AY524979, from Microbe Inst., Chinese Academy of Sciences.
Archaeal dna polymerase is the Pyrobest archaeal dna polymerases of precious bioengineering Co., Ltd, or NEB companies
Phusion archaeal dna polymerases, active unit are 5U/ μ l.
PCR cycle condition is:
94 degree of 2 minutes (pre-degeneration stages)
94 degree 20 seconds, 58 degree 20 seconds, 72 degree of 1~6 minute (30 cyclic amplification stages)
72 degree 10 minutes (finally extending the stage)
5) DNA is purified
After reaction terminates, the above-mentioned PCR samples of 5 μ l are taken to carry out agarose electrophoresis detection, it was demonstrated that the DNA fragmentation for expanding gained is big
It is small as it is expected that as, and without miscellaneous band, carry out two-step purifying and concentration, prepare DNA sample for conversion below.
The first step is to utilize PCR purification kits (being purchased from Omega companies), is carried out to specifications.Usually 50 μ l bodies
System, 4 pipes are done, totally 200 μ l, the final step that PCR is purified elute pillar to cumulative volume with 50 or 100 μ l TE buffer solutions.After purification
DNA, concentration is surveyed with NanoDrop instruments, the DNA total amounts being calculated are about 20 μ g.
Second step is to be precipitated the DNA of purifying with ethanol/sodium acetate/glycogen processing again.Specific practice is:It is past above-mentioned
The DNA solution for being dissolved in TE buffer solutions adds 1 μ l glycogens (20mg/ml), 100 μ l sodium acetates (3M, pH5.2) and the nothing of 1ml precoolings
Water-ethanol;- 80 degrees Celsius of refrigerators are placed to cool down 30 minutes;4 degree of centrifuges, under 14000 revs/min of rotating speed, centrifuge 10 minutes, stay
Precipitation;Precipitation is washed twice with the ethanol of 75% precooling again;Air-dried in super-clean bench;4 degrees Celsius of refrigerator storages, electricity are resuspended in before turning
10 μ l ultra-pure waters are standby.
6) prepared by competence and electricity turns
Chosen from the flat board of fresh activation starting strain (Candida sp.DC12, referring to《Microorganism journal》20(1):
88-93,1980, normal alkane fermenting and producing long-chain mixed dicarboxylic acid, can buy from Institute of Microorganism, Academia Sinica) single bacterium
Fall within 3ml liquid YPD mediums, 30 DEG C of shaking table cultures are stayed overnight, and rotating speed is 220 revs/min;2% transfers in 20ml YPD, and 30
DEG C shaking table culture, reaches 1.8 to OD600 by 220 revs/min;Bacterium solution is placed in and stands 15 minutes on ice, it is stopped growing,
4000 revs/min, 4 DEG C centrifuge 3 minutes, stay bacterial sediment;With the sterile washing of 4ml precoolings once;4000 revs/min, 4 DEG C of centrifugations
3 minutes, stay bacterial sediment;4ml TE/0.1M LiOAc are added, 150 revs/min, 30 DEG C of shaking table is interior to be vibrated 90 minutes;Add
0.1ml 1M DTT, 150 revs/min of continuation, the interior vibration of 30 DEG C of shaking table case 30 minutes;4000 revs/min, 4 DEG C centrifuge 3 points
Clock, stay bacterial sediment;4ml precooling sterilized waters are added, are washed 3 times;2ml 1M sorbierites are added, are washed 1 time, 4000 revs/min, 4 DEG C
Centrifugation 3 minutes;Supernatant is abandoned, 120 μ l sorbierites is added and hangs cell;40ul cell suspension is taken out in 1.5ml centrifuge tubes, is added
Enter the above-mentioned pcr amplification products (about 10 μ g) for being resuspended in sterilized water after purification of 5 μ l, mix, be placed in 5 minutes on ice;It is transferred to precooling
Electric revolving cup in, dry electric revolving cup, carry out electricity and turn that (electricity turns condition:The electric revolving cup of 2mm slits, voltage is 1800 volts, during electric shock
Between be 5 milliseconds);Electricity is added immediately 1ml sorbierites after turning, and suctions out and is put into 1.5ml centrifuge tube after mixing;4000 revs/min
Centrifugation 3 minutes, supernatant is abandoned, add 1ml YPD culture mediums, cultivated 2 hours in 37 DEG C of shaking table;4000 revs/min centrifuge 3 points
Clock, supernatant is abandoned, add 100 μ l YPD that thalline is resuspended, spread plate (YPD+clonNAT), be put into 30 DEG C of incubators and cultivate to list
Bacterium colony occurs.
7) resistant clones are screened
The single bacterium colony grown in above-mentioned resistant panel is inoculated into respectively in the centrifuge tube of 1ml YPD culture mediums, added
ClonNAT to final concentration of 100 μ g/ml, 220 revs/min, 30 DEG C of shaking table cultures.Grow, illustrate with resistant, it was demonstrated that
Resistant gene has been incorporated into phage gene group and played a role, and this part bacterium colony is used to verify in next step.Do not give birth to
Long bacterium colony, explanation are false positives, are equal to starting strain, stopping processing.
8) identify
The resistant clones of growth appearing above, YPD fluid nutrient medium overnight incubations are inoculated with, draw 500 μ l bacterium solutions, utilize treasured
The genome extracts kit of bioengineering Co., Ltd prepares genomic DNA, and concrete operations are carried out according to kit specification.
Using the genomic DNA of acquisition as masterplate, ACS-U and ACS-D are that primer enters performing PCR amplification, specific reaction system and reaction condition
With reference to the present embodiment 1 the 4) article.If the allele on target site is not knocked, expanded from two allelosomals
DNA fragmentation size out is the same, and a band is shown as in agarose electrophoresis.If one of allele on target site
It is knocked, the DNA fragmentation amplified from two allelosomals is in different size, and two are shown as in agarose electrophoresis
Band (see Fig. 3).The bacterium solution that resistance is positive and target site is knocked is accredited as, further through bacterium colony purifying and same procedure
Identification, obtain the long-chain biatomic acid production bacterial strain TDTC002 of the present invention.
Embodiment 2:The fermenting and producing of long-chain biatomic acid
After inclined-plane culture of the strain by routine, access 50ml first order seeds culture 16 hours, then first order seed is trained
It is foster to transfer into 500ml secondary seeds culture 16 hours.
The formula of seed culture medium:1~8g/L of yeast extract, 1~8g/L of corn steep liquor, sucrose 5~25g/L, KH2PO44~
12g/L, 0.5~4g/L of urea, 40~70g/L of weight wax, 121 DEG C sterilize 30 minutes.Wherein, sucrose and urea separately independent 110
DEG C sterilizing 20 minutes, mixing is remerged after sterilizing.
After the completion of secondary seed fermentation, transfer into 5L fermentation tanks.Fermentation tank culture based formulas:1~8g/L of yeast extract, corn
Starch 1~8g/L, sucrose 5~30g/L, KH2PO44~15g/L, urea 0.5~4g/L, KNO35~15g/L, NaCl 0.5~
2.5g/L, 121 DEG C sterilize 30 minutes.Wherein, sucrose and urea separately individually sterilize, and 110 DEG C sterilize 20 minutes, are closed again after sterilizing
And mix.Prepare 75% glucose solution in addition, 105 DEG C sterilize 20 minutes, fermentation carry out initial stage stream plus.Basal medium is
4L.At 30 DEG C with 1:0.5 ventilation volume, pH5.5~6.5 are controlled, started to add with 50ml/h speed stream after the 16th hour
12 carbon linear paraffins, fermentation time are 144-156 hours.Whole fermentation process is controlled with 10M NaOH solutions auto-feeding
PH, while dissolved oxygen is maintained at 30% by the adjustment of rotating speed.
As shown in Figure 4 and Figure 5, HPLC analysis shows starting strain DC12 and transformation bacterial strain TDTC002 ferments obtained length
Chain dicarboxylic acid product is consistent, purity (being respectively 98.5% and 98.9%) more than 98.5%.From following table as can be seen that transformation
Bacterial strain afterwards, conversion ratio are also improved.
Embodiment 3
According to the method for embodiment 2, simply substrate is changed to methyl laurate from 12 carbon linear paraffins.
Embodiment 4
According to the method for embodiment 2, simply substrate is changed to ethyl laurate from 12 carbon linear paraffins.