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Article

Microalgae Isolation and Selection for Prospective Biodiesel Production

by
Van Thang Duong
,
Yan Li
,
Ekaterina Nowak
and
Peer M. Schenk
*
Algae Biotechnology Laboratory, School of Agriculture and Food Sciences, The University of Queensland, Brisbane 4072, Australia
*
Author to whom correspondence should be addressed.
Energies 2012, 5(6), 1835-1849; https://doi.org/10.3390/en5061835
Submission received: 5 April 2012 / Revised: 1 June 2012 / Accepted: 14 June 2012 / Published: 15 June 2012
(This article belongs to the Special Issue Algae Fuel)
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Abstract

:
Biodiesel production from microalgae is being widely developed at different scales as a potential source of renewable energy with both economic and environmental benefits. Although many microalgae species have been identified and isolated for lipid production, there is currently no consensus as to which species provide the highest productivity. Different species are expected to function best at different aquatic, geographical and climatic conditions. In addition, other value-added products are now being considered for commercial production which necessitates the selection of the most capable algae strains suitable for multiple-product algae biorefineries. Here we present and review practical issues of several simple and robust methods for microalgae isolation and selection for traits that maybe most relevant for commercial biodiesel production. A combination of conventional and modern techniques is likely to be the most efficient route from isolation to large-scale cultivation.

1. Introduction

Microalgae have been considered for biodiesel production, based on their ability to grow rapidly and to accumulate large amounts of storage lipids, primarily in the form of triacylglycerides (TAG). Microalgae are a group of mostly photoautotrophic microorganisms that includes both prokaryotic and eukaryotic species. These organisms can photosynthetically convert CO2 and minerals to biomass, but some species also grow heterotrophically. Prokaryotic microalgae are cyanobacteria (blue-green algae) and eukaryotic microalgae include the nine phyla Glaucophyta, Chlorophyta, Chlorarachniophyta, Euglenophyta, Rhodophyta, Cryptophyta, Heterokontophyta, Haptophyta and Dinophyta. To date, about 2/3 of 50,000 species have been identified and are kept in collection by various algal research institutes [1]. For example, the largest collection at present is the Collection of Freshwater Algae at the University of Coimbra, Portugal, maintaining about 4000 strains and 1000 species of algae; the Culture Collection of Algae of the Göttingen University, Germany harbors 2213 strains and 1273 species of both freshwater and marine algae; the Culture Collection of Algae in the University of Texas, USA, maintains 2300 strains of freshwater species; the National Institute for Environmental Studies in Japan is keeping 2150 strains with about 700 species of freshwater and marine algae [2]; the Australian National Algae Culture Collection (ANACC) maintains about 1000 strains of microalgae which were mostly isolated from Australian waters [3]. Although algae collections are maintained for many purposes (e.g., for pharmaceutical, food, energy and industrial products), only a few hundred strains have been investigated for chemical content and very few are cultivated in industrial quantities. To date, although there is mounting interest to develop microalgal biodiesel production, the cost for microalgal biomass production is currently much higher than from other energy crops [4]. Thus, selection of an energy and cost-efficient production model could play a very important role in achieving competitive biodiesel production. This includes the selection of high lipid-producing algae, suitable farming locations, efficient cultivation and harvesting methods and oil extraction procedures. Here, we focus on the first step, the selection of suitable high lipid-accumulating microalgae strains, a process that can be compared with the early domestication of current crop plants. In alignment with this purpose, this review aims to present a practical guide to several simple and robust methods for microalgae isolation and selection for traits that maybe most relevant for commercial biodiesel production.

2. Advanced Microalgae Biodiesel Production

The developments in the biodiesel industry have progressed dramatically in recent years. Developed countries have set priorities on biodiesel fuels for the transport and mechanical industry and established a Biodiesel Board for policy making and development. The production of biodiesel in the EU has been increasing from 1.9 million tons in 2004 to 3.2 million tons in 2005 and to 4.9 million tons in 2006 [5]. In 2011, biodiesel production rose to 22.117 million tones as reported by the European Biodiesel Board (EBB); the leading biodiesel producing countries in the area include Germany, France and Spain [6]. The United States is also developing biodiesel applications in many different industries. According to the US National Biodiesel Board, biodiesel production increased from 0.016 million tons in 1999 to 0.787 million tons in 2004 [7]. Production and sales were estimated to have tripled from 2004 to 2005 and to have reached 21.73 million tons of fuel in 2008 and more than 31.5 million tons in 2011, as reported by The U.S. National Biodiesel Board (TUSNBB) [8]. To date, research on biodiesel production from microalgae is enthusiastically attempted globally.
In comparison with other sources (e.g., animal fat, oleaginous grain crops and oil palm), there are remarkable advantages of biodiesel from microalgae as an alternative energy source for the future. Advantages include the following: (i) areal growth rate and oil productivity of microalgae per unit of land use are much higher than those of other biofuel crops; (ii) algae grow in a wide range of environments. Fresh, brackish and saline waters are ideal environments for growth of different algae species. Even in municipal and other types of wastewater, algae grow well by using inorganic (NH4+, NO3, PO43−) as well as organic sources of nutrients [9]; (iii) microalgae absorb CO2 photosynthetically and convert it into chemical energy and biomass. The removal of CO2 from the atmosphere (and possibly industrial flue gases) may play an important role in global warming mitigation by replacing fossil fuel emissions [9,10]. Producing 100 tonnes of algal biomass fixes roughly 183 tonnes of carbon dioxide from the atmosphere [4]; (iv) microalgae can provide raw materials for different types of fuels such as biodiesel, ethanol, hydrogen and/or methane which are rapidly biodegradable and may perform more efficiently than fossil fuels [11]; (v) products extracted from algal biomass can be used as sources for organic fertilizers or high value products, such as omega-3 fatty acids, sterols, carotenoids and other pigments and antioxidants, and could be amenable to a zero waste biorefinery concept [9]. Therefore, microalgae have been regarded as possibly the only route to sustainable displacement of high proportions of fossil oil consumption.

3. Biodiesel Conversion from Microalgae

The process of isolation and selection of algae strains needs to consider the requirements of algal oil suitable for biodiesel production. Algal lipids occur in cells predominantly as either polar lipids (mostly in membranes) or lipid bodies, typically in the form of triacylglycerides. The latter are accumulated in large amounts during photosynthesis as a mechanism to endure adverse environmental conditions. Polar lipids usually contain polyunsaturated fatty acids which are long-chained, but have good fluidity properties. TAG in lipid storage bodies typically contain mostly saturated fatty acids which have a high energy contents, but, depending on the fatty acid profile of the algae strain, may lack fluidity under cold conditions. Provided the algal oil is low enough in moisture and free fatty acids, biodiesel is typically produced from TAG with methanol using base-catalyzed transesterification [12]. Most current feedstock for biodiesel production is based on plant oils produced from oil palm, soybean, cottonseed and canola, recycled cooking greases or animal fats from beef tallow or pork lard [13]. According to Fukuda, transesterification using base catalysts is 4,000 times faster than using acid catalysts [14]. Some common base catalysts used by industry are sodium hydroxide and potassium hydroxide. Use of lipase enzymes as a catalyst is efficient, however their use is limited because of the high costs [14]. The best temperature for the reaction is typically 60 °C under normal atmospheric pressure. If the temperature is higher, methanol will boil, lowering the efficiency [14]. During the transesterification process, saponification reactions can occur, forming soap. Thus, oil and alcohol must be dried. Finally, biodiesel is recovered by washing rapidly with water to remove glycerol and methanol [4]. The high potential of oil production from microalgae has attracted several companies to commercialize biodiesel from microalgae (e.g., MBD Energy Pty and Muradel Pty Ltd in Australia). Basically, algal biodiesel is produced after algae cultivation and harvesting, followed by oil extraction and its conversion by transesterification. Principally, microalgal oil can be directly used as fuel feedstock, based on the conventional process of biodiesel production, provided the fatty acid profile is favorable. But even algal oils with a high degree of saturation (e.g., similar as tallow) can be considered as a drop-in fuel (e.g., for B20 blends). In addition, scientists are also focusing on the conversion to higher value products. For example, thermal cracking is used for decomposition of triglycerides into hydrocarbons such as alkans, alkenes, and aromatic compounds [15,16].

4. Isolation and Selection Criteria for Microalgae with Potential for Biodiesel Production

4.1. Sampling and Isolation of Pure Cultures

Microalgae grow in most of the natural environments including water, rocks and soil, but interestingly also grow on and in other organisms. Their main habitats are freshwater, brackish and marine ecosystems. Microalgae can be found and collected not only in general aquatic ecosystems such as lakes, rivers and the oceans, but also in extreme environments such as volcanic waters and salt waters. Local microalgae species should be collected because it can be expected that they have a competitive advantage under the local geographical, climatic and ecological conditions. Our experience has shown that water and sediment samples from aquatic environments that undergo fluctuating and/or occasional adverse conditions provide a higher chance of isolating high lipid accumulating microalgae. Most likely these conditions would favor robust and opportunistic (fast-growing) algae with superior survival skills (e.g., by accumulation of storage lipids). Examples of these environments are tidal rock pools, estuaries and rivers.
Isolation is a necessary process to obtain pure cultures and presents the first step towards the selection of microalgae strains with potential for biodiesel production. Traditional isolation techniques include the use of a micropipette for isolation under a microscope or cell dilution followed by cultivation in liquid media or agar plates. Single cell isolation, based on traditional methods from the original sample is time-consuming and requires sterilized cultivation media and equipment, but the result of this elaborate process is always a pure culture that is usually easily identifiable. Another approach in the laboratory includes the enrichment of some microalgae strains by adding nutrients for algal growth. The most important nutrient sources for algal growth are nitrogen and phosphate. Some particular algae species may require trace minerals for their growth (e.g., silicon for diatoms). Soil water extract is an excellent source of nutrients for algae growth at this stage because this medium is easy to produce and satisfies nutrient intake of many algae strains. Although automatic isolation techniques have offered some advantages towards traditional methods (see below), single cell isolation by a micropipette (e.g., a glass capillary) is still a very effective method that can be used for a wide range of samples and is very cost-effective. An automated single cell isolation method that has been developed and widely used for cell sorting is flow cytometry [17]. This technique has been successfully used for microalgae cell sorting from water with many different algae strains [18], primarily based on properties of chlorophyll autofluorescence (CAF) and green autofluorescence (GAF) to distinguish algae species such as diatoms, dinoflagellates or prokaryotic phytoplankton.
Unlike for many agricultural crops, a targeted selection and domestication of microalgae strains is still in its infancy, while technology to economically grow microalgae with high lipid content is still being developed [4]. Each microalgae strain requires careful selection and optimization in order to increase lipid productivity with the aim to provide a cropping system with improved biofuel production and performance properties [19]. Each micro-environment may provide algae strains with very different properties. As opposed to only manipulating a few individual cultured algae strains in the laboratory for high lipid productivity, a more efficient and useful strategy to identify oleaginous microalgae would be an in-depth and systematic investigation of a whole taxonomic group of microalgae over a wide geographical and ecological distribution [20]. By correlating this with algal oil contents and optimal environmental growth conditions, a predictive tool for selecting optimal microalgae strains for biofuel production maybe developed. A bioinformatics approach could assist with the discovery of new algae isolates capable of biodiesel production and their phylogenetic grouping may suggest that potentially many more species have this ability. Typically, the steps involved in obtaining data for phylogenetic analysis include primers design (Table 1), DNA and/or RNA extraction, PCR amplification, denaturizing gradient gel electrophoresis and/or sequencing.
Table
Table 1. Examples of 18S rDNA primers for the identification of microalgae by sequencing.
Table 1. Examples of 18S rDNA primers for the identification of microalgae by sequencing.
Primer nameForward (5’–3’)Primer nameReverse (5’–3’)SpeciesReferences
TH18S5’GGTAACGAATTGTTAGTH18S3’GTCGGCATAGTTTATGThalassiosira pseudonana[21]
P45ACCTGGTTGATCCTGCCAGTP47TCTCAGGCTCCCTCTCCGGAChlorella vulgaris[22]
GTCAGAGGTGAAATTCTTGGATTTA AGGGCAGGGACGTAATCAACGDunaliella salina[23]
SS5GGTGATCCTGCCAGTAGTCATATGCTTGSS3GATCCTTCCGCAGGTTCACCTACGGAAACCNavicula sp. Chlorella sp.[24]
GAAGTCGTAACAAGGTTTCC TCCTGGTTAGTTTCTTTTCCChlamydomonas coccoides Tetraselmis suecicaNannochloris atomus[25]
CCAACCTGGTTGATCCTGCCAGTA CCTTGTTACGACTTCACCTTCCTCTNannochloropsis sp.[26]
In 2010, seven microalgae genomes had been completed [27] and current efforts to obtain many other microalgal genome sequences will enhance gene-based biofuel feedstock optimization studies (e.g., by metabolic engineering). The accumulation of storage lipid precursors and the discovery of genes associated with their biosynthesis and metabolism is a promising topic for investigation. For example, genes encoding key enzymes involved in biosynthesis and catabolism of fatty acids/TAG and their regulation are currently not well understood (for a review of the lipid biosynthesis pathway in microalgae see Schuhmann et al. [28]). By providing insight into the mechanisms underpinning the relevant metabolic processes, efforts can be made to identify molecular markers for selection or to genetically manipulate microalgae strains to enhance the production of feedstock for commercial microalgal biofuels. To date, genetic engineering approaches have been successfully used to improve biofuel phenotypes only in Chlamydomonas reinhardtii, Nannochloropsis gaditana and Phaeodactylum tricornutum [29].

4.2. Lipid Determination

Lipid determination in qualitative and quantitative analysis is crucial for identification of suitable strains for biodiesel production. Conventional methods such as solvent extraction or gravimetric methods have been used by Bligh and Dyer [30]. Separation and profiling of lipid components require elaborate techniques in order to satisfy criteria of biodiesel quality and includes thin layer chromatography (TLC), gas chromatography-mass spectroscopy (GC/MS) and/or high pressure liquid chromatography (HPLC) [31]. These methods are time-consuming for lipid extraction and analysis, especially for a large number of samples. Thus, a rapid screening for lipid content in organisms or cells is necessary and important for high-throughput screening. Nile red (9-diethylamino-5-benzo[α] phenoxazinone), a lipophilic stain, maybe used for this purpose. It was first synthesized by Thorpe in 1907 by boiling Nile blue with sulfuric acid, and in the same year, Smith reported the use of Nile red for detecting lipids in human cells [32]. The application of Nile red for lipid staining in microorganisms such as bacteria, yeasts and microalgae is now a common practice that allows a rapid qualitative determination of lipids in cells (Figure 1) [33].
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Figure 1. Cylindrotheca closterium and Scenedesmus sp. after Nile red staining under bright light (A,C) or fluorescence microscopy under blue light (B,D), respectively. Yellow dots show lipid bodies containing triacylglycerides; orange color indicates polar lipids and red shows autofluorescence from chlorophyll. Samples were obtained from a coastal rock pool (A,B); and a freshwater creek (C,D) in South East Queensland, Australia.
Figure 1. Cylindrotheca closterium and Scenedesmus sp. after Nile red staining under bright light (A,C) or fluorescence microscopy under blue light (B,D), respectively. Yellow dots show lipid bodies containing triacylglycerides; orange color indicates polar lipids and red shows autofluorescence from chlorophyll. Samples were obtained from a coastal rock pool (A,B); and a freshwater creek (C,D) in South East Queensland, Australia.
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Although Nile red can be applied for rapid lipid screening, this method has not been successful in some particular microalgae species due to variables such as staining time, temperature, rigid cell walls, etc. [34]. Thus, Nile red dye concentrations applied for lipid staining are different for particular microalgae species. To improve staining efficiency some factors can be considered. For instance, microwaves applied for staining were first introduced by Leong and Milios and then improved by Chiu et al. in 1987 [34,35,36]. Microwave exposure time was optimized for processes of pretreatment and staining. Results of this research showed that microwave-assisted staining increased remarkably fluorescence intensity using a spectrofluorometer from 476 to 820 arbitrary units (a.u.) for Pseudochlorococcum sp. and from 662 to 869 a.u. for Chlorella zofingiensis after 50 s of microwave exposure in a pretreatment process and after 60 s of staining. Dimethyl sulfoxide (DMSO) has also been used for enhancing lipid staining effectiveness [33,34,37] and maybe used in low quantities instead of acetone as a solvent to allow viability of cells after staining. This means that Nile red staining can not only be used as a preliminary quantitative fluorometric assay for relative comparisons among closely-related strains, but potentially also for mutant screening and selection of high lipid-yielding strains.

4.3. Cultivation and Biomass Production

Microalgae strains with potentially high lipid content (e.g., as determined by Nile red staining) need to be cultured to increase biomass and directly compared to each other in larger cultivation systems to assess their potential as biodiesel feedstock. Initial tests of the most promising algae strains usually are carried out at laboratory-scale using culturing flasks and other vessels, such as hanging bags, under well-defined growth conditions. The test should follow a standard protocol over a certain growth period to allow direct comparisons between strains in terms of growth rate and lipid accumulation (“lipid productivity”). It should be noted though that a standard assay does not take into consideration the potential of certain microalgae under carefully optimized conditions. An example of this assay is the following that is routinely used by our laboratory to compare lipid productivity: Pure (but not axenic) algae strains are cultured in F/2 medium (fresh or seawater) until near stationary growth occurs (less than 20% growth in 24 h as determined by cell counts). An inoculum of 5 mL of this culture is then used to start growth in 20 mL fresh F/2 medium exactly at 2 h after the start of the light cycle. The culture is then grown and monitored by cell counting for 7 days after which medium is replaced with nutrient-free water. Nutrient starvation is conducted after that for another 2 days of cultivation to test the potential for rapid TAG accumulation. In addition, biomass is collected at the end of the experiment for lipid content analysis. This assay is useful for screening of growth and lipid producing capacity of microalgae, leading to selection of potentially useful strains.
The best candidate strains with potential for biodiesel production should then be used to optimize parameters for rapid growth, lipid induction, harvesting/dewatering and oil extraction. While most of these parameters are typically optimized under small-scale laboratory conditions, it seems advisable to move towards larger size outdoor cultivation conditions as soon as possible, as these are typically quite different. Parameters, such as salinity, nutrient composition, pH and cell density can be controlled to some extent, but other factors such as temperature, irradiation and the co-cultivation of other organisms are much harder to control under outdoor conditions.
In summary, it is advantageous to isolate and screen a large number of local microalgae strains and test these under mid-scale outdoor conditions as soon as possible to be close to conditions that maybe expected for large-scale cultivation. Figure 2 provides a step-by-step overview of how microalgae may be rapidly isolated and selected for larger scale biodiesel production.

4.4. Testing at Larger Scale

At larger scale, two popular cultivation systems have been used for microalgal biomass and lipid production: open raceway ponds and closed photobioreactors. At present, open pond systems, especially large raceway ponds, are much more widely used, but bear the risk of attracting competing algae, grazers or viruses [38]. Although minimizing the cost of algae farming is one of highest priorities to achieve commercial algal biodiesel production, both systems require optimization of complex factors that satisfy high level production cultivation.
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Figure 2. Suggested 5-step protocol for rapid selection of microalgae for biodiesel production. Step 1: Local sampling sites should be chosen where microalgae frequently undergo adverse conditions; Step 2: Dilution series in growth medium provide the simplest, most cost-effective and fastest method; Step 3: Nile red staining of near stationary cultures followed by visual inspection provides a simple and rapid screening for algae with high lipid accumulation ability; Step 4: A standardized growth assay in the laboratory can provide comparative data on lipid productivity; Step 5: Parameters can be directly optimized under outdoor conditions using mid-scale cultures as these are often very different to small-scale laboratory conditions.
Figure 2. Suggested 5-step protocol for rapid selection of microalgae for biodiesel production. Step 1: Local sampling sites should be chosen where microalgae frequently undergo adverse conditions; Step 2: Dilution series in growth medium provide the simplest, most cost-effective and fastest method; Step 3: Nile red staining of near stationary cultures followed by visual inspection provides a simple and rapid screening for algae with high lipid accumulation ability; Step 4: A standardized growth assay in the laboratory can provide comparative data on lipid productivity; Step 5: Parameters can be directly optimized under outdoor conditions using mid-scale cultures as these are often very different to small-scale laboratory conditions.
Energies 05 01835 g002
For example, these include irradiation, nutrients, temperature, dissolved O2 and CO2 contents, pH, salinity, water quality, mixing efficiency and harvesting ability. Culturing and environmental conditions affect algae productivity, lipid yield and fatty acid compositions. For example, a pilot study showed that high growth rates and lipid accumulation of Chlorella sp. could be achieved primarily by increasing nitrogen concentrations and nitrogen starvation, respectively [39]. Similarly, growth of hydrocarbon-producing Botryococcus braunii was strongly dependent on light, temperature, salinity [40], nutrient quantity and composition [41]. Total lipid, carotene and chlorophyll contents of Navicula sp. increased with increasing salinity of the medium from 0.5 to 1.7 M NaCl [42]. In some cases, wastewater (e.g., municipal wastewater) can be used as a nutrient source of microalgae growth. Pulz suggested that productivity of 60–100 mg dry weight L−1 d−1 or a biomass concentration of 1 g L−1 is achievable in open pond systems [43]. Table 2 lists some of the desirable traits for the selection process of microalgae with potential for biodiesel production.
Table
Table 2. Checklist for desirable traits for microalgae selection with potential for biodiesel production and high-value byproducts.
Table 2. Checklist for desirable traits for microalgae selection with potential for biodiesel production and high-value byproducts.
StepsDesirable traits
ScreeningHigh oil
High saturated fatty acids
Low unsaturated fatty acids
High omega 3 fatty acids
Rapid and synchronized lipid production
Radiation tolerance/pigment synthesis
Antioxidants, sterols, carotenoids, astaxanthins and other pigments
Low starch contents
High protein contents
CultivationRapid growth
Salinity/freshwater tolerance
High/low temperature tolerance
Reduced antennal pigments (for improved photosynthesis in bioreactor)
Flagella properties/possession
Sheering resistance
HarvestingCell size and cell wall properties amenable for autoflocculation
Sinking speed
Foam fractionation properties
Structure and cell wall properties
ExtractionCell wall properties amenable for oil extraction
Lipid extraction efficiency

5. Lipid Content in Microalgae

Many microalgae are capable of accumulating a large amount of lipids in the cells [10]. On average, the lipid contents typically range from 10 to 30% of dry weight (Table 3). Depending on the specific algae species and their cultivation conditions, however, microalgal lipid production may range widely from 2 to 75% [2]. In some extreme cases, it can reach 70%–90% of dry weight [4,5]. For instance, the freshwater green alga Botryococcus braunii can produce oil (including hydrocarbons) up to 86% of its dry cell weight [44]. This species is being considered as a possible source for biodiesel production in the near future [4], but has the major disadvantage of slow growth rates and a low tolerance for contamination. As a result, lipid productivities (lipid production per area or volume) of other microalgae, such as Nannochloropsis, Chlorella, Tetraselmis and Pavlova sp. are typically much higher [39,45]. Lipid productivity can be dramatically increased by external application of stress factors and is considered a survival strategy for microalgae under adverse conditions. Most notably these include nutrient deprivation, exposure to chemicals, changes in salinity, temperature, pH and/or irradiation [4,39,46]. The composition of fatty acids-containing lipids differs widely among species, but, as mentioned above, generally includes structural unsaturated polar lipids, as well as neutral storage lipids, mostly in the form of TAG. Significant fatty acids used for biodiesel include saturated fatty acids and polyunsaturated fatty acids (PUFAs) containing 14–18 carbon molecules, such as C14:0, C16:0, C16:1, C18:0, C18:1, C18:2, C18:3 fatty acids [41]. According to European requirements for biodiesel standards, some fatty acids should be excluded because of undesirable properties. For instance, methyl linolenate and fatty acid methyl esters with more than four double bonds are limited to 12% due to oxidation properties [47].
Table
Table 3. Examples of lipid contents in some microalgae species [4,48].
Table 3. Examples of lipid contents in some microalgae species [4,48].
SpeciesTotal lipids (% dry weight)PUFA (% total lipids)PUFA (% dry weight)
Isochrysis galbana25.6174.3
Nanaochloropsis sp.5.62.80.2
Chaetoceros calcitrans11.88.70.9
Tetreselmis suecica2.520.90.2
Skeletonema costatum9.75.10.5
Phaeodactylum tricornutum 30
Porphyridium cruentum1.517.10.3
Crypthecodinium cohnii 20
Botryococcus braunii25.0–75.0
Chlorella sp.10.0–48.0
It is expected that microalgae that offer a multiple product portfolio as part of a biorefinery, will be most applicable to large-scale commercial cultivation. In a microalgae screening process, besides fatty acids with properties relevant for biodiesel production, some high value products such as protein-rich biomass, omega-3 fatty acids, sterols, antioxidants, vitamins and pigments should also be taken into account. In particular, omega-3 fatty acids from microalgae have received significant attention as a high-value add product, as the current sources of fish oil are unsustainable due to depleting global fish stocks. A comparison of omega-3 fatty acid contents of different microalgae shows that these differ considerably between species (Table 4).

6. Cultivation and Lipid Extraction Properties of Microalgae

High lipid productivity is not the only factor that should be considered early during strain selection. Outdoor cultivation should determine whether the selected microalgae are robust enough to withstand variable local climatic conditions and whether they can dominate a culture. This is particularly important for open pond systems where other algae strains, grazers or viruses may easily contaminate the culture. For this purpose, many phycologists recommend the use of local dominant species, even if their lipid productivity may not be as high as other species [43].
Table
Table 4. Examples of potential microalgae species for omega-3 production [48].
Table 4. Examples of potential microalgae species for omega-3 production [48].
SpeciesEicosapentaenoic acid (EPA) (% of total fatty acids)Docosahexaenoic acid (DHA) (% of total fatty acids)
Isochrysis galbana0.9
Nannochloropsis sp.30.1
Chaetoceros calcitrans34
Tetraselmis suecica6.2
Chaetoceros muelleri12.80.8
Pavlova salina19.11.5
Skeletonema costatum40.72.3
Porphyridium cruentum30.7
Crypthecodinium cohnii 30
Chroomonas salina12.97.1
Chaetoceros constriccus18.80.6
Tetraselmis viridis6.7
Harvesting capability is another important feature of microalgae with biodiesel potential. Harvesting or dewatering can be best achieved through settling, flocculation or froth flotation [49,50]. For example, many microalgae settle under adverse conditions, and this can be tested under small scale conditions [51]. Lipid extraction efficiency from microalgae is dependent on residual water content after drying and in particular the structure of their cell wall. For example, Nannochloropsis sp. is regarded a highly productive microalga with strong potential for large-scale biodiesel production [43], but ideally requires pretreatment to open up the highly rigid cell walls for higher lipid extraction efficiency.

7. Conclusions

Development of biodiesel production from microalgae presents an important move to address the limitations posed by current first generation biodiesel crops. Microalgae, once developed for commercial biodiesel production, may offer many economical and environmental advantages. Current biodiesel production from microalgae is in the research phase, but is being developed to commercial scale in many countries. Finding promising microalgae for commercial cultivation is multi-facetted and challenging because particular microalgae strains have different requirements in terms of nutrients intake, environmental and culturing conditions and lipid extraction technology. However, diversity of lipid-producing microalgae species is one of the major advantages of this group of organisms that is likely to lead to selection of suitable algae crops to achieve algal biodiesel production in different regions. A combination of conventional and modern techniques is likely the most efficient route from isolation to large-scale cultivation (Figure 2). Careful initial analyses and far-sighted selection of microalgae with a view towards downstream processing and large-scale production with potential value-add products, is an important prerequisite to domesticate and develop algae crops for biodiesel production.

Acknowledgements

We wish to thank members of the Algae Biotechnology Laboratory at The University of Queensland for their valuable comments during writing of this article, and the Australian Research Council and the Australian Endeavour Award Program for financial support.

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MDPI and ACS Style

Duong, V.T.; Li, Y.; Nowak, E.; Schenk, P.M. Microalgae Isolation and Selection for Prospective Biodiesel Production. Energies 2012, 5, 1835-1849. https://doi.org/10.3390/en5061835

AMA Style

Duong VT, Li Y, Nowak E, Schenk PM. Microalgae Isolation and Selection for Prospective Biodiesel Production. Energies. 2012; 5(6):1835-1849. https://doi.org/10.3390/en5061835

Chicago/Turabian Style

Duong, Van Thang, Yan Li, Ekaterina Nowak, and Peer M. Schenk. 2012. "Microalgae Isolation and Selection for Prospective Biodiesel Production" Energies 5, no. 6: 1835-1849. https://doi.org/10.3390/en5061835

APA Style

Duong, V. T., Li, Y., Nowak, E., & Schenk, P. M. (2012). Microalgae Isolation and Selection for Prospective Biodiesel Production. Energies, 5(6), 1835-1849. https://doi.org/10.3390/en5061835

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