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Production of biodiesel from carbon sources of macroalgae, Laminaria japonica
Xu Xu, Ji Young Kim, Yu Ri Oh, Jong Moon Park
PII: S0960-8524(14)00980-8DOI: http://dx.doi.org/10.1016/j.biortech.2014.07.015Reference: BITE 13660
To appear in: Bioresource Technology
Received Date: 5 May 2014Revised Date: 2 July 2014Accepted Date: 3 July 2014
Please cite this article as: Xu, X., Kim, J.Y., Oh, Y.R., Park, J.M., Production of biodiesel from carbon sources ofmacroalgae, Laminaria japonica, Bioresource Technology (2014), doi: http://dx.doi.org/10.1016/j.biortech.2014.07.015
This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customerswe are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, andreview of the resulting proof before it is published in its final form. Please note that during the production processerrors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.
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Production of biodiesel from carbon sources of macroalgae, Laminaria 2
japonica 3
Xu Xu a, Ji Young Kim b, Yu Ri Oh b, Jong Moon Park a,b,c * 4
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aSchool of Environmental Science and Engineering , 7
bDepartment of Chemical Engineering, 8
cDivision of Advanced Nuclear Engineering, Pohang University of Science and Technology, 9
San 31, Hyoja-dong, Pohang 790-784, South Korea 10
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* Corresponding author. 20
Tel: +82-54-279-2275; Fax: +82-54-279-8299; E-mail: [email protected] (J.M. Park) 21
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Abstract 24
As aquatic biomass which is called “the third generation biomass”, Laminaria japonica (also 25
known as Saccharina japonica) consists of mannitol and alginate which are the main 26
polysaccharides of algal carbohydrates. In this study, oleaginous yeast (Cryptococcus 27
curvatus) was used to produce lipid from carbon sources derived from Laminaria japonica. 28
Volatile fatty acids (VFAs) were produced by fermentation of alginate extracted from L. 29
japonica. Thereafter, mannitol was mixed with VFAs to culture the oleaginous yeast. The 30
highest lipid content was 48.30 %. The composition of the fatty acids was similar to 31
vegetable oils. This is the first confirmation of the feasibility of using macroalgae as a carbon 32
source for biodiesel production. 33 34
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Keywords: Laminaria japonica, Cryptococcus curvatus, Manntiol, Alginate, Volatile fatty 36
acids (VFAs), Fatty acid methyl esters (FAMEs), Biodiesel, Macroalgae 37
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1. Introduction 50
Energy problem has become one of the most serious issues all over the world since energy 51
consumption is inevitable for human existence. At this point, a large amount of alternative 52
energy appears. Among them, microbial lipids can be used as a renewable alternative 53
(biodiesel) to traditional fossil diesel fuel. Biodiesel, a mixture of fatty acid alkyl esters, can 54
be obtained from various renewable lipid resources such as vegetable oils, fats and wastes of 55
cooking oils (Liu et al., 2008). However, use of edible oils for biodiesel production competes 56
with food production and requires land and irrigation water; these requirements and the high 57
lignin content of terrestrial plants reduce the economic viability of this production mode. 58
Especially in the countries like South Korea which has no vast territory to cultivate a large 59
amount of high oil content plants, it is meaningless to use the edible oils for biodiesel 60
production. 61
On the basis of above mentioned issues, macroalgae which is called as “the 3rd generation 62
biomass” is gaining increasingly more attentions as alternative renewable sources of inputs 63
for biofuel production since it can deal with these drawbacks of terrestrial biomass and 64
produce sustainable bioenergy and materials. Macroalgae (seaweed) have several 65
advantageous characteristics such as high yield, low energy cost of production, low cost, low 66
contaminant levels and low nutrient requirements, which can be confirmed from the results 67
shown in Table 1 (Park, 2012). Macroalgae do not need land and freshwater for cultivation 68
which is advantageous to the countries lack of land. In addition, macroalgae have a lower 69
cost of the production of food and energy than other energy crops like corn and wheat. 70
Because seaweed markets are mainly existed in a few East Asian countries where seaweed is 71
utilized as food, hydrocolloids, fertilizer and animal feed (Jung et al., 2013). Macroalgae can 72
convert solar energy into chemical energy with higher photosynthetic efficiency (6-8%) than 73
terrestrial biomass (1.8-2.2%) (Jung et al., 2013). Moreover, the process of macroalgae 74
4
production introduces no contaminants, such as soil which can subsequently lead to operation 75
problems (McKendry, 2002). Comparing to the terrestrial plants, no utilization of chemical 76
fertilizers and pesticides also reduce the contaminants produced during the biomass 77
cultivation. Therefore, macroalgae have high potential as the feedstock of energy production, 78
and may be the best choice as a feedstock for biodiesel production. 79
Seaweed grows very quickly and can be harvested more than four crops per year compared 80
to the crop and forest-derived biomass which are harvested less than two crops and one crop 81
per year respectively (Table 1). Globally, about 7 million tons (wet weight) of macroalgae is 82
harvested in 2008, and the most harvested species are Laminaria japonica (sea tangle), 83
Undaria pinnatifiida (sea mustard), and Porphyra tenera (sea weed laver) (FAO, 2011). 84
According to the “Food and Agricultural Organization stats”, the highest production of 85
cultured seaweed throughout the world in 2008 was the brown seaweed, especially L. 86
japonica which was 4.8 million tons per year. Among them, L. japonica and U. pinnatifiida 87
were brown algae and L. japonica was accounted for about 65% of global production. In the 88
case of South Korea, the two most cultured species occupying around 70 % of total 89
aquaculture production are L. japonica and U. pinnatifiida. In our previous research, the 90
composition of L. japonica had been analyzed. As the data shown in Table 2, the amount of 91
carbohydrate of L. japonica is higher than that of U. pinnatifiida, which contains 60 – 67 % 92
(W/W dry). However, U. pinnatifiida has more protein (Cho, 1995). 93
In Table 3, it shows carbohydrate profile in brown algae. The two species of brown algae 94
mainly consists of alginate, laminaran, fucoidan (Kim et al., 1995, Pyeun et al., 1977). 95
Alginate and mannitol are the main structure and storage compound which account for about 96
50% (W/W) of total carbohydrates respectively (Kloareg and Quatrano, 1988). 97
Mannitol, a sugar alcohol equivalent to mannose, is one of the major carbon sources of 98
brown algae. It is different from terrestrial biomass storing carbon source as cellulose, 99
5
hemicellulose and lignin. Since cellulose is very difficult to be hydrolyzed and lignin cannot 100
be used in biorefinery, it is required high costs of pretreatment for these compounds, which is 101
the obstacle for commercialization of energy production from the terrestrial biomass. 102
However, as mannitol is soluble and available carbohydrate, it can be directly utilized by 103
microorganisms as carbon source. Alginate, the most abundant polysaccharide in L. japonica, 104
is one of brown algae’s cell wall compounds with cellulose, fucoidan, and protein (Kloareg et 105
al., 1986). The cells are strengthened to the algal tissue by both mechanical strength and 106
flexibility of alginate (Andresen et al., 1977). In the L. japonica, there are two kinds of uronic 107
acids linking each other which are polymannuronate and polyguluronate. The polymers 108
accumulate in blocks and bind divalent metal ions through forming gels which are structural 109
parts of algae. Therefore, it is less available to contact with alginate lyase. Since it is a 110
polysaccharide, the microbial oil production using alginate would require extra 111
saccharification or anaerobic fermentation process (Wang et al., 2013). Alginate has been 112
used as a food additive for a long time. Its uses are based on the properties of thickening, 113
gelling, film formation, stabilizing and general colloidal properties (Aliste et al., 2000). These 114
properties are useful in pie, cake, ice cream, and canned food productions, which can reduce 115
moisture retention, thicken batter and extend the shelf life. 116
It is well known that the first step of anaerobic digestion is hydrolysis which breaks down 117
biopolymers to monomers. In this step, carbohydrates, proteins and lipids are respectively 118
transformed into sugars, amino acids and fatty acids. These small molecules are fermented to 119
carbon dioxide and hydrogen along with several organic acids in the next step called 120
acidogenesis (Angenent et al., 2008). The organic acids produced during the acidogenesis can 121
be used by some microorganisms as carbon sources. Therefore, based on the processes 122
introduced above, L. japonica was chosen as the most appropriate substrate in this study 123
which has more carbohydrates than U. pinnatifida. 124
6
As one of the most important renewable energy sources, biodiesel is produced through 125
transesterification of vegetable oils or animal fats with short chain alcohols. However, high 126
cost of raw materials for biodiesel production has become one of the major obstacles for wide 127
application. Recently, it is gaining more attention to search for new oil sources for biodiesel 128
production. Among them, microbial oils, also known as single cell oils (SCOs), can 129
overcome these problems. In fact, all microorganisms can synthesize lipids, but only those 130
which can produce more than 20% lipids of their dry biomass are called “oleaginous” 131
including bacteria, fungi, and yeasts (Li et al., 2006, Meng et al., 2009). The oleaginous 132
yeasts possess higher specific growth rate than molds and algae, which can be considered as 133
favorable microorganisms for microbial lipids production (Li et al., 2007). The most 134
productive oleaginous yeasts are Yarrowia lipolytica, Cryptococcus curvatus, and 135
Rhodosporidium toruloides. They could produce from 40 % to 70 % of biomass (Ratledge 136
and Cohen, 2008). The microbial lipids mainly consist of triacylglycerols (TAGs), and other 137
components are free fatty acids, other neutral lipids, sterols and polar fractions (Fakas et al., 138
2006). The TAGs produced by oleaginous yeasts are mostly formed of C14 to C18 fatty acids 139
which can be used as biofuel because they are similar to vegetable oils (Li et al., 2007, Meng 140
et al., 2009). 141
C. curvatus, an oleaginous yeast, is able to accumulate up to 60% oils by dry cell weight 142
(DCW) (Ratledge, 1991) using economical carbon source . In this study, we assess whether C. 143
curvatus can be used to produce significant quantities of lipids from mannitol and alginate 144
extracted from L. japonica. 145
Because mannitol is water-soluble whereas alginate is not, a stepwise process was used 146
(Fig. 1): first, alginate was fermented under anaerobic condition to obtain VFAs which can be 147
used by C. curvatus, then the VFAs were mixed with mannitol and then added to the lipid-148
producing fermentor. It was the first time to produce lipid by oleaginous yeast only using the 149
7
L. japonica as the sole carbon source without adding any other nutrients. 150
151
2. Materials and Methods 152
2.1. Feedstock 153
Dried kelp, Laminaria japocia, was purchased from Geumil-do Fisheries Cooperation 154
Association (Wando, South Korea), milled to fine powder, and kept in a sealed container at 155
room temperature until it was used. For the trials, 90 g of the powder was mixed in 3 L tap 156
water to make the concentration 30 g/L and stirred for 6 h at room temperature to maximize 157
mannitol recovery rate in the supernatant (based on results of preliminary work), then left 158
unstirred to allow solids to precipitate. After 24 h, the mixture had separated into two layers. 159
The supernatant (~2 L) was mannitol solution; the bottom layer (~1 L) was mainly alginate 160
suspension. The supernatant was aspirated off and steam autoclaved at 121 °C for 20 min. 161
The alginate suspension was used for VFA production. 162
In the case of feedstock for lipid production, the effluent from the alginate fermentation 163
was recovered, centrifuged for 10 min at 400 g-force, and then passed through a 1.20-µm 164
filter (GF/C, Whatman, UK) to separate the liquid and solid components. The liquid part was 165
then steam autoclaved at 121 °C for 20 min. 166
167
2.2. Inoculum 168
Anaerobic digester sludge from a wastewater treatment plant (Daegu, Korea), screened 169
through a sieve (No. 10, diameter: 2 mm), then pretreated by heat at 90 °C for 20 min to 170
inactive methanogens (Lee et al., 2008). First, populations of VFA-producing bacteria were 171
increased and adapted to conditions in a 7 L fermentor (Biotron LiFlus GR Fernmentor) 172
under anaerobic condition. Heat-treated sludge (1.5 L) and 2.5 L of ground kelp (4 L working 173
volume) were added to the fermentor. It was operated at 35 °C and stirring rate was 200 ppm. 174
8
After enrichment and adaptation, the 4 L content of the fermentor was poured into a 7 L 175
continuous stirred tank reactor (CSTR) (Biotron LiFlus GR Fernmentor). Ground kelp mixed 176
with tap water (30 g/L) was supplied to the reactor under anaerobic condition using peristaltic 177
pumps (model No. 7523-30, 7521-57, Masterflex®, USA). The continuous process was 178
operated at 4 d hydraulic retention time with 2.78 mL/min flow rate. After inoculation, the 179
fermentor was purged using N2 gas for 10 min, and all instruments were maintained in strictly 180
anaerobic condition. The pH was controlled at 7 by an automatic pH controller (Model KB-181
250, K&B) using 5 M NaOH (Samchun) and 1 M HCl (Samchun) solution because this pH 182
yielded the highest VFA production rate in a preliminary study. Temperature and stirring rate 183
were maintained at 35 °C and 200 rpm respectively. Ultimately, the effluent from the CSTR 184
was directly used as the inoculum for alginate fermentation. 185
C. curvatus (ATCC 20509) was obtained from the Korean Collection for Type Culture and 186
pre-cultured in a medium composed of 1 g/L peptone, 1g/L yeast extract, and 10 g/L 187
dextrose. C. curvatus was grown in 250 mL Erlenmeyer flasks containing 50 mL of medium 188
and incubated at 28 °C in a rotary shaker which was set to 150 rpm. Before inoculation, seed 189
cells were sub-cultured for 24 h in a medium that contained 10 g/L mannitol, 1 g/L peptone, 190
and 1g/L yeast extract. The initial pH was 7.2 and the inoculum rate was 10% (v/v). 191
192
2.3. Culture conditions 193
Alginate fermentation and lipid production were conducted sequentially (Fig. 1). All 194
instruments and reactors for lipid production were steam autoclaved before use. All batch 195
tests were conducted in triplicate. 196
For VFA production from alginate, a 1.5-L fermentor (Biotron LiFlus GR) containing 1 L 197
alginate feedstock (Section 2.1.1) was seeded with 10 % (v/v) inoculum derived from the 198
CSTR effluents, then purged using N2 gas for 10 min. pH was controlled at 7 by an automatic 199
9
pH controller (Model KB-250, K&B). Temperature was maintained at 35 °C and the 200
fermentor was stirred continuously at 400 rpm. 201
For lipid production by C. curvatus, a 5-L fermentor (Biotron LiFlus GR) was utilized 202
(Fig. 1). It was loaded with 2 L of mannitol supernatant and 1 L VFAs. The pH was 203
controlled at 5.5 by an automatic pH controller (Model KB-250, K&B). Lipid production was 204
aerobic, so air was supplied at 0.5 VVM using an aerator. Temperature was maintained at 205
30 °C and the fermentor was stirred continuously at 400 rpm. 206
207
2.4. Analytical method 208
2.4.1. Physico-chemical analytical method 209
Total solid (TS), volatile solid (VS), total suspended solid (TSS), volatile suspended solid 210
(VSS) and total nitrogen (TN) were measured according to the standard method (APHA-211
AWWA-WEF, 1998). Every soluble sample was passed through a 0.45-µm pore 212
polyethersulfone syringe filter (Millipore, USA) to remove insoluble particles. 213
Mannitol, VFAs and ethanol concentrations were analyzed using a high performance liquid 214
chromatography (HPLC, Agilent Technology 1100 series) equipped with a carbohydrate-215
analysis column (Aminex HPX-87H, BIORAD INC., USA), refractive index detector (RID) 216
and diode array detector (DAD). The eluent was 0.004-M H2SO4 and the flow rate was 217
0.6 mL/min. The column temperature was maintained at 50 °C. All liquid samples were 218
diluted (1:5 or 1:10) with water and passed through a 0.2 µm syringe filter (Millipore, USA). 219
220
2.4.2. Determination of dry cell weight 221
For the dry cell weight (DCW) of C. curvatus was measured by forcing a known volume of 222
cell suspension sample through a pre-dried, pre-weighed 0.45-µm nitrocellulose filter 223
(Millipore, USA) using a vacuum pump. The samples were dried to constant weight at 224
10
110 °C in an oven, then weighed. 225
226
2.4.3. Lipid extraction 227
The extraction of total cellular lipid was performed according to Bligh and Dyer (Bligh and 228
Dyer, 1959) with modifications (Bourque and Titorenko, 2009). Lipid was extracted from 229
lyophilized biomass using a mixture of chloroform and methanol (2:1 v/v). The mixture was 230
centrifuged to partition the lipids into the solvent, then the solvent was evaporated using a 231
Nitrogen Evaporation System (Organomation Associates Inc., USA). Lipid content was 232
represented as a percentage of dry cell weight (%, W/W). Lipid concentration was defined as 233
the amount of extracted cellular lipid in per liter working volume (g/L). 234
235
2.4.4. Fatty acid methyl esters 236
The fatty acid compositions of the lipid produced by C. curvatus were determined by 237
analysis of fatty acid methyl esters (FAMEs). The FAMEs were produced by 238
transesterification: methanol was added to the extracted lipid with sulfuric acid (2.5 % V/V 239
H2SO4/CH3OH) as a catalyst; the reaction was allowed to proceed for 45 min at 90 °C. Then 240
1 ml H2O and 2 ml n-hexane were added. The FAMEs dissolved into the n-hexane. The 241
solution was centrifuged at 2000 rpm for 15 min, to separate the water from the 242
FAME/hexane phase which was then transferred into glass vials using Pasteur pipettes. 243
The FAMEs in n-hexane were analyzed using a gas chromatography (6890N, Agilent, 244
USA) equipped with a flame ionized detector (FID) and an INNOWAX capillary column 245
(Agilent, USA, 30 m × 0.32 mm × 0.5 µm). The column temperature was programmed as 246
follows: (1) initial column temperature 100 °C, hold for 5 min, (2) increase to 250 °C at 247
10 °C/min, hold for 30 min. The split ratio was 1:10 (v/v). The injector and the detector 248
temperatures were both set at 250 °C. FAME components were identified and quantified by 249
11
comparing the retention times and peak areas with those of standard solutions. 250
251
3. Results and discussion 252
3.1. VFA production by alginate fermentation using mixed cultivation system 253
As mentioned in the materials and methods, the inoculum of alginate fermentation was the 254
effluent from a CSTR. In fact, the CSTR was a VFA-producing system which can 255
continuously produce acetate, propionate and butyrate using L. japonica as sole carbon 256
source without adding any other nutrients. This system has been operated for over 1000 d in 257
our previous research and stabilized more than 600 d. Therefore, the microbial community in 258
the effluent from the CSTR was quite stable. 259
To evaluate the profile changes of acids during alginate fermentation, mannitol 260
consumption along with the accumulation and consumption of acidogenic products in batch 261
reactor were demonstrated (Fig. 2). Although the mannitol and alginate were separated by 262
natural sedimentation, the liquid (mannitol solution) could not be completely separated from 263
the solid (alginate suspension). Therefore, liquid samples for HPLC analysis after 264
centrifugation retained some mannitol (5.8 g/L initially). The products of alginate 265
fermentation were acetate, succinate, lactate, formate, acetate, propionate, butyrate and 266
ethanol. Ethanol concentration reached 1.0 g/L within 24 h, but gradually decreased to 0 by 267
144 h, probably because ethanol initially produced was converted into acetate by 268
acidogenesis (Angenent et al., 2008). The depletion of ethanol and production of acetate are 269
thermodynamically favorable (Oh et al., 2003). Likewise, succinate, lactate and formate also 270
increased to a certain amount and disappeared later. During the period of acidogenesis, 271
acetate was produced as a major alginate fermentation product, followed by propionate and 272
butyrate. The final concentration of acetate was more than 9.0 g/L at 6.5 d. Propionate 273
concentration slowly increased to 3.5 g/L, and remained at that level until 156 h. Butyrate 274
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was produced until 24 h and its concentration began to increase from 36 h, ultimately to a 275
concentration which was more than 0.5 g/L. At the end of digestion, the VFAs consisted of 276
69.2 % acetate, 25.7 % propionate and 5.1 % butyrate. 277
278
3.2. Cell growth and lipid accumulation by C.curvatus using carbon source derived from 279
macroalgae by single batch cultivation system. 280
Most of the microorganisms can synthesize lipids, but only the oleaginous strains may 281
accumulate more than 20 % W/W lipids on dry cell basis (Papanikolaou and Aggelis, 2011a). 282
Microorganisms synthesize lipids by either de novo processes that utilizes hydrophilic 283
substances as substrates, or by ex novo processes that utilize hydrophobic substances as 284
substrates. In this research, all lipid synthesis occurred by de novo processes. In de novo 285
processes, lipid accumulation always happens after depletion of nitrogen (or to a lesser extent 286
of other essential nutrient like phosphorus or sulfate) from the medium (Papanikolaou and 287
Aggelis, 2011b). In addition, to ensure that VFAs are mostly converted into lipids rather than 288
to biomass, these carbon sources should be added to a medium containing enough cells 289
(Fontanille et al., 2012). 290
Total nitrogen (TN) was 134 mg/L in the mannitol supernatant and 48 mg/L in the VFA 291
effluent. Initially 1 L of VFA effluent was added to the 2 L of mannitol substrate; this 292
addition diluted manntiol and VFA concentration in the substrate to 2/3 and 1/3 of pre-293
addition levels, respectively. During the first 12 h, VFAs were not dramatically consumed by 294
C. curvatus. Lipid concentration and DCW increased slightly at the same time. However, 295
lipid content increased rapidly from less than10 % to 30 %. During the next 36 h, lipid 296
content, lipid concentration, and DCW increased to a much higher level until 48 h when all 297
VFAs were used up by yeasts. As for lipid content, it achieved its highest point (48.30%). It 298
is obvious that the concentration of mannitol was almost constant until 48 h, which could 299
13
demonstrate that in lipid-producing metabolic pathway of C. curvatus, VFAs were more 300
preferable than mannitol as a carbon sources under pH of 5.5. After the exhaustion of VFAs, 301
mannitol began to gradually decrease and was consumed up within 84 h. In the meantime, 302
DCW increased to 3.60 g/L until 72 h and then remained stable; whereas lipid content 303
suddenly reduced which resulted in the decrease of lipid concentration. This phenomenon 304
which is called as “lipid turnover” is related with storage lipid degradation (Chen et al., 2012, 305
Peng et al., 2013). Microbial lipid turnover has been extensively studied in Y. lipolytic and C. 306
echinulata (Papanikolaou and Aggelis, 2011a). Oleaginous yeasts consume their own 307
intracellular lipids to maintain lipid-free biomass when carbon source is exhausted or carbon 308
uptake rate decreases. Because there was still some mannitol left in the substrate, the lipid 309
turnover could result from the reduced carbon source uptake rate. When VFAs were 310
exhausted, C. curvatus had to consume mannitol as substitution, which could make the 311
carbon source uptake rate decreased during this process. From 72 h, lipid content increased 312
again with more mannitol assimilated by the yeasts. 313
Several research groups have used VFAs to produce lipids by culturing oleaginous yeasts 314
including Yarrowia lipolytica and Cryptococcus curvatus (Christophe et al., 2012, Fontanille 315
et al., 2012). The most significant difference was that in our study the microorganisms 316
utilized mannitol and VFAs which were all derived from seaweed without addition of any 317
other nutrients and reagents, whereas in other research, oleaginous yeasts used a synthetic 318
medium containing glucose and acetate as substrates. Moreover, in other research the ratio of 319
carbon to nitrogen (C/N) was artificially controlled by continuously adding carbon and 320
nitrogen sources to achieve high lipid concentration and content. But in our work, we just 321
utilized the original mannitol supernatant and alginate fermentation effluents to culture the 322
oleaginous yeasts. 323
We compared our results to other researches that also used VFAs or acetate as carbon 324
14
sources (Table 4). In fact, little research has examined the feasibility of using mannitol as a 325
carbon source for oleaginous yeasts. In addition, the strains and concentration of carbon 326
source used were all different with each research. Therefore, the only relevant comparisons 327
was of the value of lipid content (% W/W). Among these results, apparently the lipid content 328
in this work (48.30%) was higher than that of any other researches. It indicated that the 329
mannitol and VFAs derived from alginate anaerobic fermentation were favorable for 330
microbial lipid production even without using synthetic medium or artificially adding any 331
other nutrients. 332
333
3.3. Fatty acid composition analysis 334
The fatty acids produced in our study consisted mainly of palmitic acid (C16:0), stearic 335
acid (C18:0), oleic acid (C18:1), and linoleic acid (C18:2) (Table 5). Others indicates C8:0, 336
C10:0, C12:0, C14:0, C16:1, C18:3, C20:0, C20:1, C20:2, and C24:0. This composition is 337
similar to those of vegetable oils which have been utilized for industrial production of 338
biodiesel (Adamska ET, 2004). Over time, some changes in lipid composition occurred. 339
Obviously, there were three different trends shown in each fatty acid composition. As for 340
C18:0 and C18:1, they both increased during the period of VFAs consumption until 48 h, 341
while the percentages decreased when C. curvatus started to assimilate mannitol as the sole 342
carbon source. In contrast, in the case of palmitic acid, it was gradually reduced during the 343
first 48 h, then accumulated again until the end. However, the profile of linoleic acid 344
followed a totally different pattern. The percentage increased throughout the period from 345
8.95 % to 17.15 %, irrespective of which carbon source yeasts used. This composition was 346
comparable to vegetable fatty acids indicating that the fatty acids accumulated by C. curvatus 347
are appropriate for use in biodiesel production (Li et al., 2007, Meng et al., 2009). 348
349
15
4. Conclusions 350
We designed an efficient batch system for lipid production by the oleaginous yeast 351
Cryptococcus curvatus using two different carbon sources derived from a brown macroalga, 352
Laminaria japonica: mannitol and VFAs obtained by anaerobic fermentation of alginate with 353
a mixed culture. This is the first demonstration of microbial oil production by bioconversion 354
of macroalgae without addition of any other carbon sources or nutrients. This study has 355
shown that mannitol and VFAs derived from alginate fermentation are favorable feedstock 356
for lipid production. Future work can focus on optimizing and scaling up this process. 357
358
Acknowledgements 359
This research was supported by Basic Science Research Program through the National 360
Research Foundation of South Korea (NRF) funded by the Ministry of Education, Science 361
and Technology (Grant number 2011-0001108), the Advanced Biomass R&D Center (ABC) 362
of South Korea Grant funded by the Ministry of Education, Science and Technology (ABC-363
2011-0028387), Marine Biotechnology Program Funded by Ministry of Land, Transport and 364
Maritime Affairs of South Korean Government, South Korea and the Manpower 365
Development Program for Marine Energy funded by Ministry of Land, Transportation and 366
Maritime Affairs (MLTM) of South Korean government and by the World Class University 367
(WCU) program through the National Research Foundation of South Korea funded by the 368
Ministry of Education, Science and Technology (R31-30005). 369
370
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459
460 461
18
Figure legends: 462 463
Fig. 1. Schematic diagram of alginate fermentation and lipid production processes. 464
465
Fig. 2. Profile of various carbon sources and volatile suspended solid (VSS) variations 466
during the alginate fermentation. (▲) VSS; (◇) mannitol; (○) acetic acid; (▼) 467
propionic acid; (□) butyric acid; (◆) ethanol; (ⅹ) formic acid; (▽) lactic acid; (△) 468
succinic acid. 469
470
Fig. 3. Profile of mannitol (◇), acetic acid (○), propionic acid (▼), butyric acid (□), 471
dry cell weight (DCW)(●), lipid concentration (▲), lipid content (■) during a two-step 472
batch cultivation of Cryptococcus curvatus in a 5 L fermentor. 473
19
Table 1. Comparisons between 1st, 2
nd, and 3
rd generation biomass
Resourcea Crop Forest-derived Seaweed
Harvesting 1 – 2 /yr 1 / 8yr 4 – 6 /yr
Production (ton/ha) 180 9 565
CO2 uptake (ton/ha) 5 – 10 4.6 36.7
Energy yield (%) 30 - 35 20 – 25 > 45
Cost ($/L) 0.2 – 0.3 0.4 0.2
a (Park, 2012)
20
Table 2. Composition of Laminaria japonica and Undaria pinnadifida
(% w/w, dry base) Protein Lipid Ash Carbohydrate
Laminaria japonica 6.8 – 10.3 7.2 – 11.5 13.8 – 21.1 60.9 – 67.0
Undaria pinnadifidaa 13.7 – 28.7 3.6 – 6.2 29.4 – 46.5 26.5 – 42.8
a (Cho, 1995)
21
Table 3. Characteristic algal polysaccharides in Laminaria japonica and Undaria pinnadifida
Algal carbohydrate (% w/w, dry base)
Alginate Fucoidan Laminaran Mannitol Total
Laminaria japonica 14.6 – 29.5 0 – 0.1 3.7 – 4.2 22.5 – 33.2 40.8 – 67.0
Undaria pinnadifidaa 22.3 – 32.9 1.4 3.6 4.1 – 7.3 31.4 – 45.2
a (Kim et al., 1995, Pyeun et al., 1977)
22
Table 4. Lipid production by oleaginous yeasts using different substrate in two-step system
Strains Carbon source (g/L) DCW (g/L) Lipid conc. (g/L) Lipid content (% W/W) Reference
C. albidus VFAs (2.00) 1.16 0.31 27.00 (Fei et al., 2011a)
C. albidus Acetate (6.00) 2.85 0.74 25.80 (Fei et al., 2011b)
Y. lipolytica Acetate (12.00) 5.98 1.84 30.76 (Fontanille et al., 2012)
C. curvatus Mannitol + VFAs (9.30) 3.60 1.30 48.30 This study
a Calculated based on references.
23
Table 5. Fatty acid methyl ester (FAME) profile of C. curvatus
Fermentation time (h)
Fatty acid methyl ester (FAME) profile of C. curvatus (%)
Palmitic AME (C16:0)
Stearic AME (C18:0)
Oleic AME (C18:1)
Linoleic AME (C18:2)
Othersa
0 25.88 12.83 48.16 8.95 4.18
12 25.62 11.64 48.36 10.65 3.73
24 21.16 15.45 49.38 11.41 2.60
36 14.72 22.41 50.34 11.49 1.05
48 14.70 19.46 52.26 12.78 0.80
60 15.33 18.20 52.13 13.29 1.06
72 16.75 15.76 49.31 16.32 1.86
84 18.18 14.03 48.71 17.15 1.93
a Others: C8:0, C10:0, C12:0, C14:0, C16:1, C18:3, C20:0, C20:1, C20:2, and C24:0.
24
Fig. 1. Schematic diagram of alginate fermentation and lipid production processes.
Mannitol Supernatant
Alginate Slurry
Lipid Fermentor
AeratorFlow Meter pH Controller
VFAs
Alginate Fermentor
pH Controller
Substrate
(30 g/L Laminaria japonica)
25
Fig. 2. Profile of various carbon sources and volatile suspended solid (VSS) variations during alginate fermentation. (▲) VSS; (◇)
mannitol; (○) acetic acid; (▼) propionic acid; (□) butyric acid; (◆) ethanol; (ⅹ) formic acid; (▽) lactic acid; (△) succinic acid.
Time (h)
0 24 48 72 96 120 144
Co
nce
ntr
ati
on
(g
/L)
0
2
4
6
8
10
12
VS
S (
g/L
)
0
10
20
30
40
26
Fig. 3. Profile of mannitol (◇), acetic acid (○), propionic acid (▼), butyric acid (□), dry cell weight (DCW)(●), lipid concentration
(▲), lipid content (■) during a batch cultivation of Cryptococcus curvatus in a 5 L fermentor.
Time (h)
0 12 24 36 48 60 72 84
DC
W, M
an
nit
ol a
nd
VF
As (
g/L
)
0
2
4
6
8
10
Lip
id c
on
cn
. (g
/L)
0.0
0.5
1.0
1.5
2.0
Lip
id c
on
ten
t (%
)
0
10
20
30
40
50
27
H I G H L I G H T S
▶This is the first demonstration of microbial oil production by using macroalgae.
▶Oleaginous yeast Cryptococcus curvatus was used for microbial oil production.
▶Carbon sources were all derived from Laminaria japonica.
▶No addition of any other nutrients or synthetic medium was used.
▶The composition of the fatty acids was found similar to vegetable oils.