APPLIED AND ENVIRONMENTAL MICROBIOLOGY, Oct. 2009, p. 62226231 0099-2240/09/$08.00 0 doi:10.1128/AEM.01162-09 Copyright 2009, American Society for Microbiology.

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Vol. 75, No. 19

Poly(3-Hydroxybutyrate) Production from Glycerol by Zobellella denitricans MW1 via High-Cell-Density Fed-Batch Fermentation and Simplied Solvent Extraction
Mohammad H. A. Ibrahim and Alexander Steinbuchel*
Institut fur Molekulare Mikrobiologie und Biotechnologie, Westfalische Wilhelms-Universitat Munster, 48149 Munster, Germany
Received 19 May 2009/Accepted 28 July 2009

Industrial production of biodegradable polyesters such as polyhydroxyalkanoates is hampered by high production costs, among which the costs for substrates and for downstream processing represent the main obstacles. Inexpensive fermentable raw materials such as crude glycerol, an abundant by-product of the biodiesel industry, have emerged to be promising carbon sources for industrial fermentations. In this study, Zobellella denitricans MW1, a recently isolated bacterium, was used for the production of poly(3-hydroxybutyrate) (PHB) from glycerol as the sole carbon source. Pilot-scale fermentations (42-liter scale) were conducted to scale up the high PHB accumulation capability of this strain. By fed-batch cultivation, at rst a relatively high cell density (29.9 1.3 g/liter) was obtained during only a short fermentation period (24 h). However, the PHB content was relatively low (31.0% 4.2% [wt/wt]). Afterwards, much higher concentrations of PHB (up to 54.3 7.9 g/liter) and higher cell densities (up to 81.2 2.5 g/liter) were obtained by further fed-batch optimization in the presence of 20 g/liter NaCl, with optimized feeding of glycerol and ammonia to support both cell growth and polymer accumulation over a period of 50 h. A high specic growth rate (0.422/h) and a short doubling time (1.64 h) were attained. The maximum PHB content obtained was 66.9% 7.6% of cell dry weight, and the maximum polymer productivity and substrate yield coefcient were 1.09 0.16 g/liter/h and 0.25 0.04 g PHB/g glycerol, respectively. Furthermore, a simple organic solvent extraction process was employed for PHB recovery during downstream processing: self-otation of cell debris after extraction of PHB with chloroform allowed a convenient separation of a clear PHB-solvent solution from the cells. Maximum PHB recovery (85.0% 0.10% [wt/wt]) was reached after 72 h of extraction with chloroform at 30C, with a polymer purity of 98.3% 1.3%.

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Polyhydroxybutyrate (PHB) is the best-studied example of biodegradable polyesters belonging to the group of polyhydroxyalkanoates (PHAs), which are synthesized by many bacteria and archaea as intracellular carbon and energy reserves (1, 40, 43). In the last decades, these biopolymers have received great attention due to their properties which resemble those of conventional petrochemical-based polymers (49). For instance, PHB is very similar to thermoplastic polypropylene (17). Their production from renewable resources and their complete biodegradability give PHAs promising advantages from an environmental point of view (6). In addition to their special physical traits, such as the elasticity of medium-chainlength PHAs and the high crystallization rate of PHB, PHAs are biocompatible, water resistant, oxygen impermeable, and enantiomerically pure; all of these characteristics broaden the scope of their applications in industry and medicine. So far, higher production costs than those of petrochemical plastics have hindered the successful commercialization of PHB (9). Many efforts have been devoted to reducing the production costs by developing superior microbial strains ca-

* Corresponding author. Mailing address: Institut fur Molekulare Mikrobiologie und Biotechnologie, Westfalische Wilhelms-Universitat Munster, Corrensstrasse 3, D-48149 Munster, Germany. Phone: 49 251-8339821. Fax: 49-251-8338388. E-mail: steinbu@uni-muenster.de. Published ahead of print on 7 August 2009. 6222

pable of utilizing cheap substrates and also by applying more efcient fermentation strategies and economical recovery processes (10). Fed-batch fermentation regimens are usually applied to achieve a high cell density, which is necessary for a high productivity and yield, in particular in cases of intracellular products, by frequent or continuous feeding of nutrients when growth proceeds (46). Several fed-batch fermentation processes have been reported for PHA production (21, 28). There are two prevalent cultivation modes for PHB production that are imposed on the microorganisms being used. The more frequently used mode is realized by a complex two-stage cultivation process. In this mode, all nutrients needed for growth to a high cell density are provided during the rst phase of the process. In the second phase, imbalanced growth conditions are enforced by providing growth-limiting amounts of nutrients such as nitrogen, phosphate, or oxygen to trigger PHA biosynthesis and accumulation. The model organism for this mode is Ralstonia eutropha (formerly known as Alcaligenes eutrophus and recently reclassied as Cupriavidus necator) (26, 27). In the other cultivation mode, PHB is accumulated concurrently with growth, and therefore a single-stage process is applicable. A well-known example of this mode is PHB production by Alcaligenes latus (18, 47). Although several new downstream processes for the extraction of PHA have been reported as being economically effec-

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tive, such as the application of surfactants and hypochlorite (9, 38), dispersions of hypochlorite solution and chloroform (14, 15), and the selective dissolution of cell mass by proteolytic enzymes (25) or by sulfuric acid and hypochlorite (48), solvent extraction methods are still regarded as an adequate way to gain intact polymers with a high purity and recovery yield (39). However, there is still a need to develop and improve these extraction methods further to make the entire process much simpler and cheaper (22). In addition to increased prices for crude oil, the abundance of inexpensive raw materials from agriculture and industry as cheap substrates for microbial fermentations, such as crude glycerol from the biodiesel industry, could make the production of PHA from renewable resources more competitive with common plastics (32). Due to increased glycerol production by the growing biodiesel industry, the prices for glycerol became low enough to make this residual compound a cheap carbon source for several industrial fermentation processes, especially for the production of microbial polyesters (11, 34). However, the various amounts of actual fermentable substrates and the presence of other nonfermentable components in feedstock, such as the various concentrations of glycerol and salts in biodiesel coproducts, hinder their use (42). Therefore, tolerant bioprocesses and/or strains tolerant to such variable factors are required. The production of PHA from glycerol has been investigated in only a few studies (4, 12, 24, 33, 42). In a recent study (32), crude glycerol from different biodiesel manufacturers was examined for suitability as a substrate for PHB production. However, signicant decreases in PHB productivity and product yields were recorded when NaCl-contaminated crude glycerol was used. Recently, a newly isolated bacterium, Zobellella denitricans MW1, was characterized as producing large amounts of PHB from glycerol, with enhanced growth and polymer productivity in the presence of NaCl (20). The present study aimed at developing a strategy to improve the volumetric production of PHB by Z. denitricans MW1, using glycerol as the sole carbon source. For this purpose, several fed-batch cultivations were set up to steadily improve the nutrient supply to attain a high cell density and high PHB productivity. Moreover, the conventional organic solvent extraction method was modied with regard to an economically more feasible large-scale PHB extraction, achieving a high purity and recovery of the polymer.
MATERIALS AND METHODS Microorganism and culture conditions. Z. denitricans strain MW1, a recently isolated and characterized bacterium accumulating PHB from glycerol (20), was used in this study. Cells were grown in mineral salt medium (MSM) (41) containing the following (g/liter): Na2HPO4 12H2O, 9.0; KH2PO4, 1.5; MgSO4 7H2O, 0.2; NH4Cl, 1.0; CaCl2 2H2O, 0.02; and Fe(III)NH4 -citrate, 0.0012. The MSM also included 1 ml of trace element solution containing the following (g/liter): EDTA, 50.0; FeCl3, 8.3; ZnCl2, 0.84; CuCl2 2H2O, 0.13; CoCl2 6H2O, 0.1; MnCl2 6H2O, 0.016; and H3BO3, 0.1. Glycerol (15 g/liter) was used as the sole carbon source. The pH was adjusted to 7.3 before sterilization. MSM with 15 g/liter agar was used as a solid medium for maintenance of the bacterium at 4C. Precultures were grown in 250-ml and 2-liter Erlenmeyer asks containing 50 and 400 ml MSM, respectively. The asks were incubated at 41C and 200 rpm for 24 h. Cultivation at 42-liter scale. A Biostat UD-30 stainless steel reactor (B. Braun Biotech International, Melsungen, Germany) with a total volume of 42 liters (28-cm inner diameter and 71-cm height) and a d/D value relation (relation of

stirrer diameter to vessel diameter) of 0.375 was used for cultivations at the 30-liter scale. This bioreactor was equipped with three stirrers, each containing six paddles and a Funda-Foam mechanical foam destroyer (B. Braun Biotech International, Melsungen, Germany). In addition, sterilized probes were inserted into ports to measure dissolved oxygen (pO2) (model 25; Mettler Toledo GmbH, Steinbach, Switzerland), pH (model Pa/25; Mettler Toledo GmbH), foam (model L300/Rd. 28; B. Braun Biotech International), temperature (pt 100 electrode; M. K. Juchheim GmbH, Fulda, Germany), and optical density at 850 nm (OD850) (model CT6; Sentex/Monitek Technology Inc.). The operations were controlled and recorded by a digital control unit in combination with the MFCS/win software package (B. Braun Biotech International). Cultivations were done at 41C and at a pO2 between 0 and 100% saturation in the medium, which was controlled by agitation rates between 100 and 800 rpm and aeration rates between 0.4 and 1.67 volume per volume per minute. Unless stated otherwise, the pH in the medium was held between 7.0 and 7.3 by controlled addition of 4 N HCl or NaOH. Foam was removed by a mechanical foam destroyer; if this was not sufcient, the antifoam agent Silikon Antischaum Emulsion SLE (Wacker, Darwin Vertriebs GmbH, Ottobrunn, Germany) was added. Small samples were withdrawn from the culture uid for analytical purposes. Cell harvest from 42-liter cultivations. Cells were harvested by centrifugation in a CEPA type Z41 or type Z61 continuous centrifuge (Carl Padberg Zentrifugenbau GmbH, Lahr, Germany). Harvested cells were frozen at 30C and then lyophilized (Beta 1-16; Christ, Osterode, Germany). Determination of cell growth. Growth of Z. denitricans MW1 was monitored by measuring the increase of the OD600. Moreover, dened volumes of cultures were harvested by centrifugation for 20 min at 1,200 g and 4C; afterwards, the cells were washed with distilled water, frozen, and lyophilized. Cell density, dened as the cell dry weight (CDW) per liter of culture broth, was determined by weighing aliquots of lyophilized cells. Fluorescence microscopy. The presence of cytoplasmic PHA inclusions was evidenced by staining the biopolymer with Nile red and by observing the cells under a uorescence microscope (30). PHB extraction from Z. denitricans MW1 whole cells. Small-scale solvent extraction experiments were done to investigate the extraction efciencies of different organic solvents for optimum PHB recovery from Z. denitricans MW1 cells. One hundred milligrams of lyophilized cells was mixed overnight at room temperature with 20 volumes of different solvents (chloroform, methylene chloride, carbon tetrachloride, diethyl ester, ethyl acetate, and mixtures of chloroform and acetone [1:1, 1:2, 1:3, 1:4, 2:1, 3:1, and 4:1] [vol/vol]) in 2-ml sealed glass tubes. After extraction, cells were separated by otation or precipitation, depending on their behavior in the solvent being used. PHB was recovered after solvent evaporation. Larger-scale solvent extraction experiments were done by stirring 100 g of lyophilized cells in 1,000 ml chloroform or methylene chloride (10 volumes) at a temperature of 24, 30, or 41C. Samples of 50 ml were withdrawn after different incubation periods lasting up to 228 h. Before ltration, samples were left overnight in separation funnels until complete otation of cells had occurred, thereby yielding a clear PHB-solvent solution for easy and simple ltration. After ltration, the PHB-solvent solutions were concentrated by distillation (solvent recovery), and 2 to 4 volumes of cold methanol was used to precipitate the PHB. Afterwards, the precipitated PHB was ltered and dried under vacuum. Analyses of ammonium and glycerol. The concentrations of ammonium in cell-free supernatants were determined by employing a gas-sensitive type 152303000 ammonium electrode (Mettler Toledo GmbH, Greifensee, Switzerland). Analysis of residual carbon sources was carried out with a LaChrom Elite high-performance liquid chromatography apparatus (VWR-Hitachi International GmbH, Darmstadt, Germany) consisting of a Metacarb 67H advanced C column (Bio-Rad Aminex equivalent; Varian, Palo Alto, CA) and a VWRHitachi model 22350 column oven. The column (300 mm by 6.5 mm) consisted of a sulfonated polystyrene resin in the protonated form. The primary separation mechanism included ligand exchange, ion exclusion, and adsorption. A VWRHitachi refractive index detector (type 2490) with an active-ow-cell temperature control and automated reference ushing eliminating temperature effects on the refractive index baseline was used for detection. Aliquots of 20 l were injected and eluted with 0.005 N sulfuric acid in double-distilled water at a ow rate of 0.8 ml/min. Online integration and analysis of the data were done with EZ Chrome Elite software (VWR International GmbH, Darmstadt, Germany). Quantitative analyses. To determine the PHB contents of the cells, samples were subjected to methanolysis in the presence of 15% (vol/vol) sulfuric acid. The resulting 3-hydroxybutyric acid methyl esters were analyzed by gas chromatography (GC) (19). PHB content (% [wt/wt]) was dened as a percentage of CDW. The purity of extracted PHB was also determined by GC from a known

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IBRAHIM AND STEINBUCHEL

APPL. ENVIRON. MICROBIOL.

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FIG. 1. Fed-batch cultivation of Z. denitricans for PHB production from glycerol in the absence of NaCl (fed-batch 1). Z. denitricans MW1 was cultivated in a Biostat UD-30 stirred-tank reactor containing 24 liters of MSM with glycerol as the sole carbon source. The bioreactor was inoculated with 4% (vol/vol) 18-h preculture. The pO2 was controlled automatically at 30% saturation by adjusting aeration and agitation rates. Cells were grown for 24 h at 41C and pH 7.3. During the time course of cultivation, samples were withdrawn, and the concentrations of glycerol and ammonium, as well as the cell density and the PHB content of the cells, were determined as described in Materials and Methods.

mass of solvent-extracted PHB. The percentage of PHB recovered was calculated from a known amount of PHB in the biomass, based on the purity of the total mass of samples recovered. The substrate conversion factor (g PHB/g glycerol) was calculated as grams of PHB produced per grams of glycerol utilized. All results are from duplicate or triplicate measurements, and mean values and standard deviations are presented.

RESULTS Production of PHB by fed-batch cultivation of Z. denitricans MW1. Four fed-batch fermentations at the 42-liter scale were carried out to obtain high cell densities and high polymer contents of cells of the newly isolated bacterium Z. denitricans MW1, using glycerol as the sole carbon source. In accordance with the results of a previous study done with small Erlenmeyer asks (20), cultivation temperature and pH were controlled at 41C and 7.3, respectively. In the rst fermentation (Fig. 1), an overnight seed culture was used to inoculate 24 liters of MSM (4% [vol/vol] inoculum size). Feeding was started after 6 h of batch culture, using a 50% (vol/vol) solution of glycerol. The dissolved oxygen (pO2) level in the medium was controlled automatically at 30% by increasing the agitation and aeration rates to 800 rpm and 1.67 volume per volume per minute, respectively. The feeding regimen was designed to provide sufcient amounts of glycerol (10 to 20 g/liter) to support both cell growth and polymer accumulation during growth of Z. denitricans MW1. Ammonium chloride solution (25% [wt/vol]) was added if the ammonium concentration in the culture fell below 1.0 g/liter. The specic growth rate ( ) during the batch phase was 0.09/h, and the maximum specic growth rate recorded was 0.351/h, with a doubling time of 1.97 h. At the end of this fermentation (24 h), a high cell density and also high volumetric polymer productivity were obtained (29.9 1.3 g CDW/ liter and 9.28 1.7 g PHB/liter, respectively). However, the

PHB content was relatively low (31.0% 4.2% [wt/wt]). The two main problems which prevented the extension of this fermentation to reach higher cell densities and polymer contents were the excessively added NaOH solution to control the sharp decrease in pH during the last 6 hours of this fermentation, which should cause signicant cell lysis, and the increased medium volume because of nutrient feeding and base addition. The total amount of 4 kg glycerol used yielded a total of 0.33 kg PHB, thereby indicating a low substrate conversion factor of 0.10 0.02 g PHB/g glycerol. Fed-batch fermentation in the presence of NaCl. In the next fed-batch fermentations (batches 2, 3, and 4) (Table 1), the reported enhancing effect of sodium chloride on growth and polymer accumulation (20) was investigated on a large scale (42 liters). In addition, some modications in the feeding strategy were conducted. A 24-h-old preculture (800 ml) with approximately 3 g CDW/liter was used to inoculate 20 liter MSM containing 15 g/liter glycerol. The total amount of sodium chloride for 30 liters (600 g) was added at the beginning of the fermentation. The feeding solution used contained 1% (wt/vol) MgSO4 and 50% (vol/vol) glycerol. The pO2 was kept at 20% saturation. Culture pH was controlled at 7.3 during the rst 20 h of growth and then at 6.8 until the end of fermentation, using sodium hydroxide (4 N) and ammonia water (25% [wt/ vol]); the latter was also used as a nitrogen source, as well as NH4Cl (25% [wt/vol]). In fed-batch 2, a similar cell density (32.8 0.6 g CDW/liter) to that of fed-batch 1 was reached, in spite of using only half the amount of glycerol (Table 2). The relatively optimized cultivation conditions resulted in a higher polymer content of 52% 1.4% (wt/wt), producing 17.1 0.8 g PHB/liter after 36 h of cultivation. The product yield was improved to 0.26 0.01 g PHB/g glycerol.

VOL. 75, 2009

PHB PRODUCTION FROM GLYCEROL TABLE 1. PHB production by Zobellella denitricans MW1 in fed-batch fermentationsa

6225

Fed-batch fermentation no.

Initial vol (liters)

Final vol (liters)

Cultivation time (h)

Amt of glycerol (g)

Residual amt of glycerol (g)

CDW (g/liter)

% PHA (wt/wt)

PHA concn (g/liter)

PHB productivity (g/liter/h)

Yield (g PHB/g glycerol)

1 2 (NaCl) 3 (NaCl) 4 (NaCl)

24 20 20 20

36 26 33 30

24 36 63 50

4,059 2,100 5,725 8,400

768 360 250 1,884

29.9 32.8 63.9 81.2

1.3 0.6 2.0 2.5

31.0 52.0 56.0 66.9

4.2 9.3 1.4 17.1 0.7 35.8 7.6 54.3

1.7 0.8 1.6 7.9

0.39 0.47 0.57 1.09

0.07 0.02 0.02 0.16

0.10 0.26 0.22 0.25

0.02 0.01 0.01 0.04

a Fed-batch fermentations were done by cultivating Z. denitricans MW1 in a 42-liter Biostat UD-30 stainless steel reactor. Medium components, feeding solutions, and cultivation conditions were as described in the text. All fermentations were operated at 41C. Fed-batch fermentations 2, 3, and 4 were supplied with 20 g/liter NaCl. Analyses were done in triplicate, and averages and standard deviations are presented.

Using these improved results, further optimizations were done using the same fed-batch technique, but with increased amounts of glycerol and ammonia. Aiming to reach a higher cell density despite the lack of information available for the recently isolated Z. denitricans strain MW1, nutrient requirements for cell growth were estimated according to the general calculation method for bacteria (13). In the third fed-batch fermentation (Fig. 2), the same feeding solution used in fedbatch 2 was supplemented with trace elements, iron, and calcium, providing two times their original concentrations in MSM during the entire time course of the fermentation. The total estimated amounts of glycerol and ammonia were fed to keep concentrations of 10 to 20 g/liter of glycerol and 1 to 2 g/liter of ammonium. In this fed-batch fermentation, signicant increases in cell density (195%) and volumetric PHB productivity (201%) compared to those in fed-batch 2 were obtained using a semicontinuous feeding regimen, which provided adequate carbon and nitrogen for growth and polymer accumulation over a period of 63 h. In addition, the polymer content increased slightly, to 56% 0.7% (wt/wt), and the PHB productivity increased substantially, to 0.57 0.02 g/ liter/h. The substrate conversion factor was kept higher than 0.2 g PHB/g glycerol. In the last fed-batch fermentation (fed-batch 4) (Fig. 3), a higher cell density and polymer content were targeted while keeping the satisfying product yield obtained during the previous fed-batch cultivations. The concentration of glycerol in the feeding solution was increased to 80% (vol/vol). NH4OH (25% [wt/vol]) was used in parallel with NaOH (4 N), instead of ammonium chloride solution, for improved control of the pH of the medium and also to provide enough nitrogen for growth. On the basis of ofine analytical data (high-performance liquid chromatography analysis of the glycerol concentration in samples withdrawn from the bioreactor), the feeding rate was increased or decreased if necessary during continuous feeding to keep the glycerol concentration between 10 and 20 g/liter. The maximum growth rate and doubling time were 0.422/h and 1.64 h, respectively. The highest cell density achieved was 81.2 2.5 g CDW/liter, and the maximum OD600 obtained was 351 5.3. In addition, a high PHB content (66.9% 7.6% [wt/wt]) was reached after a relatively short fermentation time (50 h), thereby enhancing the polymer volumetric productivity up to 54.2 7.9 g PHB/liter, with an improved product yield (0.25 0.04 g PHB/g glycerol). In summary, during this fed-batch fermentation (30-liter nal volume), 2.44 kg CDW containing 1.63 kg PHB was produced from 6.52 kg glycerol. Growth-associated PHB accumulation

was monitored microscopically. Figure 3C shows the increased prevalence of PHB granules inside Z. denitricans MW1 cells during fed-batch fermentation 4. Extraction of PHB from Z. denitricans MW1 cells. In this study, extraction of PHB from cells of Z. denitricans MW1 was investigated by different methods, such as the use of detergents or decolorizing agents, dispersion of cells in hypochlorite solution and chloroform, and the selective dissolution of cell mass by sulfuric acid and hypochlorite. However, the degree of purity obtained by these methods was very low in comparison to the purity of PHB prepared by solvent extraction (data not shown). Many problems were faced during separation of non-PHB cell materials or during residual hypochlorite wash-off steps, in addition to an excessive need for high-speed centrifugation. These problems would be magnied in the large-scale extraction process for PHB and would require special precautions, especially if highly viscous PHB-solvent solutions were employed. During the search for a simple but perfect recovery of PHB from Z. denitricans MW1 cells, different organic solvents were investigated in small-scale experiments (100 mg cells in 2 ml organic solvent) to determine their efciency in recovering PHB and how easy the separation of PHB from cell debris after extraction could be. Only chloroform and methylene chloride showed remarkable efciencies in PHB recovery. No detectable PHB was extracted from the cells with carbon tetrachloride, diethyl ester, ethyl acetate, or mixtures of chloroform and acetone under the conditions studied (data not shown). Self-occulation and otation of Z. denitricans MW1 cells were recorded for carbon tetrachloride, chloroform, and methylene chloride, whereas in diethyl ester and ethyl acetate the cells settled down. On the other hand, oating/settling priority in chloroform-acetone mixtures depended on the prevalence of chloroform, i.e., if the percentage of chloroform was less than 75% (vol/vol), then the cells would sediment. Because of their PHB extraction efciencies, chloroform and methylene chloride were selected for large-scale experiments (100 g cells in 10 volumes solvent) to optimize PHB extraction from Z. denitricans MW1 cells with a high recovery and efcient oating. The data in Table 3 show the effects of incubation temperature and time on the efciency of solvent recovery of PHB. At room temperature (24C), chloroform recovered 54.5% 0.06% (wt/wt) of the PHB from the cells after 24 h of extraction. Extending the extraction time to up to 228 h was not correlated with an increase in the amount of recovered polymer. However, the chloroform extraction efciency increased signicantly when incubation was done at a higher

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TABLE 2. Overview of literature describing production of PHAs from glycerol by bacteria

Mediuma Type of PHA PHB PHB PHB 17.00 0.254 0.17 13.50/8.40 0.223 0.17 4 4 37 5.07.5% Gly, 3% Cas-Pep or Cas A 30 37 40 60 67/45 1232 47/65 30 45 2122 50 Cultivation temp (C) PHA content (% wt/wt ) PHA concn (g/liter) Cultivation time (h) Cell density (g CDW/ liter) PHA productivity (g/liter/h) Yield (g PHA/g substrate) Reference

Bacterium

Cultivation vessel, fermentation strategy

2.5-liter bioreactor (batch)

2.5-liter bioreactor (batch)

IBRAHIM AND STEINBUCHEL

Flask culture

5.07.5% Gly, 3% Cas-Pep or Cas A BM, 0.5% YE, 0.5% Pep, 1% Gly

250-ml ask

BM, 0.5% YE, 0.5% Pep, 1% Gly

37

48

60

PHB

4.80

0.100

31

500-ml ask 30 30 72/96 1.9, 3.4 40, 20 72 2.1 42 mcl-PHA

Medium E,b 15% CSBP 30 72 1.3 1327 PHB

0.170.35 0.88

0.0020.005 0.012

2 2

500-ml ask

500-ml ask (P. oleovorans incubated for 24 h before addition of P. corrugate and then 48 or 72 h of mixed incubation) 42-liter fed-batch culture 1% GLP, 2.5% YE, 2.5% Pep MBM, 0.25% Try, 0.1% YE, 3% Gly MYA, 3% Gly SGA, 35 41 41 0.5% Gly 37 60 3050 after nitrogen limitation 96 50 37 48 30 34 0.310.45 15.3 21.17 2225 5 81.2 37 182 21.3 76 31.440.7 51.9 51 70/48 87 66.9

Medium E,b 1% CSBP Medium E,b 15% Gly

s/mcl-PHA blends

0.97, 0.67

PHBV (810 mol% HV) PHB PHB PHB PHB PHB PHB

16.20 0.100.17 7.90 10.81 12.00 4.27 54.32

0.090 0.0030.005 0.200 0.180 0.1600.240 0.044 1.090

0.23

24 7 0.08 12 33 0.37/0.14 0.29 0.25 32 20 This study

1,000-ml ask

5.6-liter bioreactor (batch)

5.6-liter fed-batch culture

Methylobacterium rhodesianum MB126 Ralstonia eutropha DSM 11348 Recombinant E. coli JM109 harboring genomic DNA fragment from Streptomyces aureofaciens NRRL 2209 Recombinant E. coli (ATCC PTA-1579) harboring Streptomyces aureofaciens PHB biosynthesis genes Pseudomonas oleovorans NRRL B-14682 Pseudomonas corrugate 388 Mixed culture of Pseudomonas oleovorans NRRL B-14682 and Pseudomonas corrugate 388 Unidentied osmophilic organism Vibrio sp. isolates M11, M14, M20, and M31 Recombinant E. coli strain with PhaPc Recombinant E. coli arcA mutant Cupriavidus necator JMP 134

2-liter fed-batch culture

Zobellella denitricans MW1

250-ml ask

42-liter fed-batch culture

MSM, 1% Gly, 1% crude Gly (ADM 5.5% NaCl ) MSM, 1.5% Gly, 2% NaCl MSM, 1.5% Gly, 2% NaCl

APPL. ENVIRON. MICROBIOL.

a CSBP, coproduct steam from soy-based biodiesel production (1% CSBP has 2.3 g available glycerol); GLP, glycerol liquid phase from biodiesel production (70% wt/wt glycerol); YE, yeast extract; Try, tryptone; Cas, casein; Cas A, Casamino Acids; Gly, glycerol; Pep, peptone; SGA, Sabouraud glucose agar medium; MBM, marine basal medium; BM, basal medium; ADM, ADM Hamburg AG (biodiesel manufacturer). b See reference 5. c Granule-associated protein from Azotobacter sp. strain FA8.

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FIG. 2. Fed-batch cultivation of Z. denitricans for PHB production from glycerol in the presence of NaCl (fed-batch 3). Z. denitricans MW1 was cultivated in the presence of NaCl in a Biostat UD-30 stirred-tank reactor containing 20 liters of MSM with glycerol as the sole carbon source. A total of 2% NaCl was added at the beginning of the fermentation. The fermenter was inoculated with 4% (vol/vol) 24-h preculture. The pH of the medium was controlled at 7.3 during the rst 20 h of growth and then at 6.8 until the end of fermentation, using NaOH (4 N) or NH4OH (25% [wt/vol]). The glycerol feeding solution (50% [vol/vol]) was supplemented with 1% MgSO4 and two times the normal concentrations of trace elements, iron, and calcium in MSM. The pO2 was controlled automatically at 20% saturation by adjusting aeration and agitation rates. Cells were grown for 63 h at 41C. During the time course of cultivation, samples were withdrawn, and the concentrations of glycerol and ammonium, as well as the CDW and PHB content of the cells, were determined as described in Materials and Methods.

temperature. At 30C, 74.2% 0.09% (wt/wt) of the PHB was recovered from the cells after 24 h. The maximum recovery rate, 85.0% 0.10% (wt/wt) of PHB, with a purity of 98.3% 1.3%, was achieved after 72 h by use of 10 volumes of CHCl3 at 30C. Figure 4 shows the complete otation of cells in a separation funnel after 16 h of incubation at room temperature. A slightly lower recovery rate (81.7% 0.09% [wt/wt]) and purity (97.9% 0.8%) were detected after 120 h. The latter may be due to excessive cell lysis during a prolonged incubation time, which may hinder otation of cell debris. Increasing the temperature during chloroform extraction to 41C did not enhance the recovery efciency, since low PHB recovery (65.9% 0.08%) and low purity (94.2% 2.5%) were observed in comparison to those reached at 30C. Also, at high temperature, increased cell lysis resulted in a very low oating velocity of cell debris, and after 48 h of extraction at 41C, cells could not be separated by otation. Extraction with methylene chloride yielded a lower recovery rate than that attained with chloroform. For instance, after 24 h, only 32.6% 0.04% (wt/wt) of the PHB could be recovered from the cells at 24C; this is only about 60% of the PHB recovered by chloroform for the same temperature and incubation period. PHB recovery by methylene chloride was only marginally enhanced by increasing the extraction time to 72 h (Table 3). DISCUSSION Production of PHB from glycerol by the recently isolated bacterium Z. denitricans MW1 was scaled up by using the fed-batch fermentation mode at the 42-liter scale. In the rst

fed-batch fermentation, a relatively high cell density and high polymer productivity were achieved after a short incubation time (24 h). Both were higher, by factors of 8.5 and 13.4, respectively, than those recently recorded in ask-scale experiments after 96 h (20). In spite of the low PHB content and the low product yield reached in this fed-batch cultivation experiment, the cell density and also the PHB content and product yield were comparable to the data published for the production of PHB from glycerol (Table 2). A slightly lower product yield (0.080 g PHB/g glycerol) was recorded for recombinant E. coli strains in 5.6-liter batch fermentations (12). A similar cell density was also reported for a recombinant arcA mutant of E. coli in a 5.6-liter fed-batch culture (33). A higher PHB content (76% [wt/wt]) was achieved by an unidentied osmophilic organism in a 42-liter fed-batch fermentation using glycerol liquor phase with yeast extract and peptone. However, the productivity was very low (0.09 g/liter/h) because of the long cultivation time (182 h) (24). Several ask-scale cultivations were carried out with a variety of bacterial strains, such as a recombinant E. coli strain harboring PHB synthesis genes from Streptomyces aureofaciens (31, 37), different Pseudomonas strains (2, 3), and several Vibrio sp. isolates (7), but only comparably low PHA productivities were attained. Batch culture of R. eutropha DSM 11348 in a 2.5-liter fermenter with glycerol and casein peptone or Casamino Acids resulted in the maximum productivity (0.254 g/liter/h) reported for PHB production from glycerol (4). Signicant decreases in PHB content (from 70 to 48% [wt/ wt]) and also in product yield (from 0.37 to 0.14 g/g) were recorded for PHB production by Cupriavidus necator JMP 134 using NaCl-contaminated crude glycerol (5.5% [wt/vol] NaCl)

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VOL. 75, 2009 TABLE 3. Solvent extraction of PHB from Z. denitricans MW1 cellsa
Solvent (temp) Time (h) Amt of extracted PHB (g/50 ml solvent) Recovery (%) Purity (%)

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Chloroform (24C)

24 48 72 228 24 48 72 96 120 24 24 48 72 228

1.82 1.84 1.85 1.81 2.47 2.81 2.83 2.82 2.72 2.19 1.09 1.13 1.21 1.05

0.04 0.04 0.06 0.03 0.10 0.03 0.13 0.12 0.21 0.05 0.03 0.03 0.10 0.03

54.5 55.4 55.6 54.4 74.2 84.3 85.0 84.7 81.7 65.9 32.6 34.1 36.2 31.5

0.06 ND 0.06 ND 0.06 97.6 2.1 0.06 96.8 1.8 0.09 ND 0.10 ND 0.10 98.3 1.3 0.10 ND 0.09 97.9 0.8 0.08 94.2 2.5

Chloroform (30C)

Chloroform (41C) Methylene chloride (24C)

0.04 ND 0.04 ND 0.04 98.8 1.0 0.04 96.4 2.7

a Lyophilized cells of Z. denitricans MW1 (100-g portion) from fed-batch fermentation 4 (66.9% 7.6% PHB wt/wt ) were stirred into 10 volumes of solvent at different extraction temperatures. Fifty-milliliter sample portions were withdrawn at the indicated times. Samples were separated in separation funnels overnight at room temperature. Clear PHB-solvent solutions were withdrawn and concentrated. Afterwards, 4 volumes of methanol was added to precipitate PHB, which was then ltered and dried under vacuum. Recovery and purity of PHB were analyzed by GC. Analyses were done in triplicate, and averages and standard deviations for three different analyses are presented. ND, not determined.

(32), which might be related to the increased osmotic pressure caused by NaCl accumulation during glycerol feeding. This problem can be ignored if halophilic bacteria or moderate halophiles are used under such conditions. On the other hand, some of these bacteria have been studied for PHB productivity (16, 36), but the need for additional salts for strain requirements elevated the production costs (29, 40) and could further accelerate the corrosion of commonly used stainless steel fermenters (8, 35). In this respect, further optimizations of fed-batch fermentations by Z. denitricans MW1 were made by utilizing the reported enhanced growth and polymer content in the presence of sodium chloride (20). First, the modied feeding and pH control improved the product yield to 260%, since half the amount of glycerol (1.74 kg) was utilized, producing 445.4 g PHB with a higher polymer productivity (0.47 0.02 g/liter/h). Further optimizations of fed-batch fermentation with increased feeding rates of glycerol and ammonia, together with

the precise control of pH, maximized PHB productivity, to 1.09 0.16 g/liter/h, with a higher polymer content (66.9% 7.6% [wt/wt]) and a high product yield (0.25 0.04 g PHB/g glycerol), which is the highest yield reported so far for the production of PHA from glycerol (Table 2). Although Z. denitricans MW1 accumulates PHB during growth, slightly increased PHB contents were detected at a low concentration of ammonium chloride (20). Therefore, a short nale of limited nitrogen conditions was provided in all fedbatch fermentations (batches 1, 2, 3, and 4) for enhanced polymer accumulation. An increased PHB content after applying the nitrogen limitation condition was also reported for growth-associated PHB accumulation by A. latus during batch and fed-batch cultures (45). As shown in Fig. 3A, the ofine direct control feeding regimen used has some critical points, such as the drop in glycerol concentration to 5 g/liter at 12 and 29 h, and also the ammonia concentration decreased to 0.17 g/liter at 43 h. At the same time that glycerol was depleted (12 and 29 h), an increase in pO2 was detected (Fig. 3B), and this could be a basis for the application of indirect control of glycerol concentration in further optimization. However, precise direct control of glycerol is also anticipated to maximize cell density and polymer productivity. High PHB productivity from glucose (2.42 g/liter/h) was achieved by a glucose-utilizing mutant of A. eutrophus H16 when a direct online glucose control was applied compared to the productivity reached with pH state for a fed-batch (0.25 g/liter/h) of the same strain (23). Also, for higher-cell-density cultivation, a pure oxygen supply is a signicant concern, since the maximum stirring and airow used in fed-batch 4 could not provide enough dissolved oxygen in the exponential growth phase (up to 36 h) (Fig. 3B). Due to its physicochemical characteristics, glycerol as a substrate will pose a challenge in oxygen transfer rates as well. Eventually, ease of recovery of PHA is a very important parameter for economically feasible production of the polyester (22). In this respect, otation of Z. denitricans MW1 cells after solvent extraction is considered the easiest way to achieve a cell-free PHB-solvent solution by an in situ separation step, avoiding additional costs for centrifugation and waste of polymer during recovery steps. The highest recovery rate was reached with chloroform at 30C after 72 h. Recently, another method of selective dissolved-air otation for PHA recovery from cell debris of Pseudomonas putida was also investigated (44). A slightly lower recovery and purity were reported for the extraction of PHB from A. eutrophus by chlorinated solvent

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FIG. 3. PHB production by Z. denitricans MW1 during continuous feeding of glycerol (fed-batch 4). Cultivation was done in a Biostat UD-30 stirred-tank reactor containing 20 liters of MSM with glycerol as the sole carbon source. A total of 2% NaCl was added at the beginning of the fermentation. The bioreactor was inoculated with 4% (vol/vol) 24-h preculture. (A) Glycerol was fed continuously to keep its concentration higher than 10 g/liter. The glycerol feeding solution (80% [vol/vol]) was supplemented with MgSO4 (1% [wt/vol]) and two times the normal concentrations of trace elements, iron, and calcium in MSM. During the time course of cultivation, samples were withdrawn, and the concentrations of glycerol and ammonium, as well as the CDW and PHB content of cells, were determined as described in Materials and Methods. (B) The following parameters were obtained by online monitoring: OD850, pO2 (controlled automatically at 20% saturation by adjusting aeration and agitation rates), and the pH of the medium (controlled at 7.3 during the rst 20 h of growth and then at 6.8 to the end of fermentation, using NaOH [4 N] and NH4OH [25% {wt/vol}] in parallel). Fermentation was operated for 50 h at 41C. (C) Microscopic photographs showing the accumulation of PHB granules in cells during the entire time course of fermentation (9, 14, 24, 32, 45, and 50 h). The left panels (with size bars) show pictures obtained by phase-contrast light microscopy of cells possessing bright cytoplasmic inclusions. The right panels (without size bars) show uorescence micrographs of PHB inclusions stained with Nile red.

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IBRAHIM AND STEINBUCHEL

APPL. ENVIRON. MICROBIOL.

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FIG. 4. Flocculation and otation of Z. denitricans MW1 cells in separation funnels after extraction of PHB with chloroform. This experiment was done with 200 g lyophilized cells in 2 liters of CHCl3. (A) Cell-PHB-chloroform mixture directly after extraction. (B) Floating cell layer on top of clear PHB-chloroform solution after overnight incubation at room temperature.

reux (39). In spite of the short extraction time recorded (15 min), the high temperatures (61C for CHCl3 and 40C for CH2Cl2) at which reux was done and the need for 24 h of cell pretreatment with acetone should hinder the application of this recovery method at the industrial scale. Compared to all other strains used for PHB production from glycerol (Table 2), this study recommends Z. denitricans MW1 as a new and attractive option for large-scale production of PHB by use of residual crude glycerol from the biodiesel industry.
ACKNOWLEDGMENTS Financial support of this study by BASF AG (Ludwigshafen, Germany) is gratefully acknowledged. We thank Yasser Elbahloul, Ahmad Sallam, Kaichien Lin, Kay Frey, and Herbert Ahlers for their assistance during fermentation.
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