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Applied and Environmental Microbiology, August 2003, p . 5029-5031, Vol . 69, No . 8

Increased Exopolysaccharide Production in Lactococcus lactis due to Increased Levels of Expression of the NIZO B40 eps Gene Cluster

Ingeborg C . Boels,1,2,{dagger} Richard van Kranenburg,1,2,{ddagger} Marja W . Kanning,2 Barrie Fong Chong,2,§ Willem M . de Vos,1 and Michiel Kleerebezem1,2*

Wageningen Centre for Food Sciences, Wageningen,1 NIZO Food Research, Ede, The Netherlands2

Received 10 March 2003/ Accepted 27 May 2003


   ABSTRACT

 
Exopolysaccharides (EPS) play an important role in the rheology and texture of fermented food products . This is the first report demonstrating that homologous overexpression of a complete eps gene cluster in Lactococcus lactis leads to increased EPS production levels . A ninefold-elevated EPS plasmid copy number led to an almost threefold increase in the eps expression level, resulting in an almost fourfold increase in the NIZO B40 EPS production level . It was previously reported that increased EPS precursor levels did not influence NIZO B40 EPS production levels . However, the present results indicate that the maximal NIZO B40 EPS production level is limited by the activity level of the expression products of the eps gene cluster rather than by the level of EPS precursors .


   INTRODUCTION

 
In the dairy industry, exopolysaccharide (EPS)-producing lactic acid bacteria (LAB) are used to improve the texture of fermented diary products . Different LAB produce a wide variety of EPS that have potential applications as food additives . These EPS would be preferable over presently used stabilizers, such as xanthan, since their production hosts have a food-grade status . However, LAB EPS are formed only at relatively low production levels (40 to 800 mg liter-1) compared to those of commercially produced EPS (10 to 25 g of xanthan liter-1) (1) . Nevertheless, some EPS produced by LAB are very effective biothickeners when produced in situ (5, 13) . Among EPS-producing LAB, one of the best characterized is Lactococcus lactis NIZO B40, which harbors a 42,180-bp EPS plasmid, pNZ4000, containing the 12-kb eps operon (14, 16) . Previously it was demonstrated that the overproduction of the NIZO B40 priming glucosyltransferase resulted in a 15% increased EPS production compared to that of the control strain (15) . These data suggest that elevation of the level of eps gene expression could result in higher EPS production .

To elevate the level of eps gene expression, we cloned the entire NIZO B40 eps gene cluster of pNZ4000 (14) on the high-copy-number vector pIL253 (10), yielding pNZ4120 . This was achieved by introducing an NcoI site with the help of a double-stranded oligonucleotide (link-F and link-R; Table 1) that was subsequently used for the cloning of the 17-kb NcoI fragment of pNZ4000, encompassing the entire eps gene cluster . Plasmid pNZ4120 was transformed into L . lactis NZ9000 (7), and the resulting strain was used to determine the relative copy number of the EPS plasmid (relative to the chromosomal DNA copy number) by using real-time PCR . Exponentially grown lactococcal cells (20 µl) were harvested by centrifugation and were disrupted by a microwave treatment (2 min, 800 W) . Disrupted cell pellets, including total DNA, were suspended in 20 µl of water and were directly used for PCRs . These reactions contained the primer pairs designed on epsC (TM-epsC-F and TM-epsC-R), pepN (TM-pepN-F and TM-pepN-R), and ery (TM-ery-F and TM-ery-R) (Table 1) and were performed by using the TaqMan core reagent kit (Applied Biosystems, Nieuwerkerk aan de Ijssel, The Netherlands) . The threshold cycle number (Ct) was determined (6) by using the ABI Prism 7700 sequence detection system software and was used to calculate the relative gene copy number (Nrelative) for each strain with the formula Nrelative = 2(CtgeneX - Ct pepN) (Table 2), with the chromosomally carried pepN gene as an internal standard of chromosomal DNA quantification . An almost ninefold higher relative EPS plasmid copy number was found in cells of strain NZ9000 harboring pNZ4120 compared to that of cells harboring the pNZ4030 plasmid, indicating that replacing its endogenous replication machinery by that of pIL253 could increase the EPS plasmid copy number significantly .


TABLE 1 . Strain, plasmids, and oligonucleotide sequences of a DNA linker, forward (F) and reverse (R) primers, and probes which contain a G-carboxyfluorescein (FAM) reporter dye and a G-carboxytetramethylrhodamine (TAMRA) quencher dye used in real-time PCR and reverse transcriptase (RT) primers used in RT-PCR

 

TABLE 2 . EPS production, DNA copy numbers of the NIZO B40 EPS plasmid, and expression levels of the eps genes of L . lactis strain NZ9000 harboring pNZ4030 or pNZ4120c

 
The effect of increased EPS plasmid copy number on the expression of the eps genes was analyzed by quantification of the relative eps mRNA level . Therefore, mRNA isolated from exponentially grown cells with the help of an RNeasy kit (Qiagen, Leusden, The Netherlands) was reverse transcribed by using Omniscript reverse transcriptase (Qiagen) and reverse transcriptase primers, which were designed on epsC (TM-epsC-RT) or pepN (TM-pepN-RT) containing a dedicated 5' tag for cDNA/DNA discrimination (12) (Table 1) . The cDNA generated was subsequently amplified by real-time PCR using the primer pairs designed on epsC (TM-epsC-F and TM-epsC-R2) and pepN (TM-pepN-F and TM-pepN-R2) . The relative expression levels of the eps genes in strain NZ9000 harboring pNZ4120 (relative to the expression level of the chromosomally located pepN gene) were almost threefold higher than those observed in the same strain harboring pNZ4000, establishing that the expression of the eps genes can be raised to a higher level by increasing the copy number of the EPS plasmid .

Overexpression of the entire eps gene cluster resulted in a significantly reduced growth rate and a lower final optical density (Table 2) . In addition, the relative carbon flux towards EPS production was threefold increased (Table 3), suggesting that increased EPS production generates a significant metabolic burden due to the required high-level production of sugar nucleotides, which are utilized in both EPS production and growth . This suggestion is supported by the observation that sugar-nucleotide pools in EPS-producing cells are lower than those of non-EPS-producing cells (8, 9) .


TABLE 3 . Carbon balance of glucose consumption and product formation in L . lactis strain NZ9000 harboring EPS plasmid pNZ4030 or pNZ4120

 
Previously it was reported that increasing the enzyme activity levels of the household genes involved in the EPS biosynthesis pathway led to increased EPS precursor levels (2, 3) . However, this did not result in increased NIZO B40 EPS production levels . In contrast, EPS production was fourfold elevated in the eps overexpression strain (Table 2), suggesting that the EPS production level could be directly correlated to the eps gene expression level . This would indicate that the maximal NIZO B40 EPS production level is limited by the activity level of the expression products of the eps gene cluster rather than by the level of sugar nucleotides . However, this hypothesis might not hold true for the biosynthesis of EPS other than NIZO B40 . The latter is supported by the findings that the level of Streptococcus pneumoniae type 3 capsular polysaccharide production in L . lactis can be dramatically increased by the expression of the pneumococcal capsular polysaccharide precursor-forming enzyme UDP-glucose pyrophosphorylase (4) .

To evaluate the effect of EPS overproduction on the biophysical properties of the fermentation broth, the kinetic viscosity of the EPS-overproducing strain was measured by using an Ubbelohde viscometer with a capillary diameter of 0.63 mm (17), and it appeared to be 1.6-fold increased relative to that of the cells producing the native EPS production level (Table 2) . These results indicate that improvement of EPS production levels positively influences the viscosity properties of the fermented product .

Here we have described the targeted analysis of an important bottleneck in EPS production . We could increase the NIZO B40 EPS production level fourfold by overexpression of the NIZO B40 eps genes in L . lactis . Furthermore, the results suggest that the EPS production level is directly correlated to the eps gene expression level and could possibly be raised even further . The identification of EPS production bottlenecks is important for future challenges for the construction of lactococcal strains that produce EPS with novel properties . The results presented here are a first step toward the development of lactococcal production hosts of EPS that could be applied as food additives .

 


   ACKNOWLEDGMENTS

 
We thank Jan van Riel for determination of EPS contents and Roelie Holleman for determination of cell metabolites .


   FOOTNOTES

 
* Corresponding author . Mailing address: Department of Flavor, Nutrition and Ingredients, NIZO Food Research, P.O . Box 20, 6710 BA Ede, The Netherlands . Phone: 31-318-659629 . Fax: 31-318-650400 . E-mail: michiel.kleerebezem{at}nizo.nl .

{dagger} Present address: Corporate Research, Friesland Coberco Dairy Foods, Deventer, The Netherlands .

{ddagger} Present address: Purac, Gorinchem, The Netherlands .

§ Present address: The University of Queensland, St . Lucia, Brisbane, Queensland 4072, Australia .


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What Is Dna?, What Is Functional Genomics?, What Is Biofilter?, What Is Fermentation?, What Is Staphylococcus Aureus?, s, Microorganisms, c, Bacteria, o, Microorganism, n, Microbiology, s, Bacteriology, r, Sepsis, c, Functional genomics, a, Escherichia coli, n, S. cerevisiae, i, Enterobacters, i, E coli O157, c, E coli O157, n, Yeasts, s, Cryptococci, n, Thermophile, s, Antibiotics, n, Pseudomonas aeruginosa, e, Bacteriological, c, Streptococcal, s, Bacillus subtilis, o, Escherichia coli, e, Erythromycin, a, Escherichia coli, a, Pathogenic bacterium, a, Multidrug resistant, n, Sepsis




 

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