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 CHEMICAL ENGINEERING TRANSACTIONS  
 

VOL. 49, 2016 

A publication of 

 
The Italian Association 

of Chemical Engineering 
Online at www.aidic.it/cet 

Guest Editors: Enrico Bardone, Marco Bravi, Tajalli Keshavarz
Copyright © 2016, AIDIC Servizi S.r.l., 
ISBN 978-88-95608-40-2; ISSN 2283-9216 

Enhanced Lipid Extraction from Microalgae Chlorella vulgaris 
Biomass: Experiments, Modelling, Optimization 

Dmitry Dvoretsky, Stanislav Dvoretsky, Mikhail Temnov, Evgeniy Akulinin, 
Evgeniya Peshkova 

Тambov State Technical University, ul. Sovetskaya 106, Tambov 392000, Russia 
dvoretsky@tambov.ru 

Microalgae are a promising raw material source for the production of lipids. However, the existing technologies 
of lipid extraction from microalgae would benefit from their improvement. The objective of the present study 
was to determine optimal conditions for lipid extraction from Chlorella vulgaris (C. vulgaris) microalgae 
biomass.  
As a result of the conducted research, a method of cell walls disruption has been selected, and types and ratio 
of polar and non-polar solvents at the extraction stage have been experimentally identified. Also, the influence 
of extraction process conditions (temperature, type, and amount of extraction solvents added per unit of 
biomass) on the degree of lipid extraction from C. vulgaris IFR №С-111 microalgae biomass has been 
determined. 
The efficiency of microalgae cell walls disruption has been compared for the following disruption methods: 
microwave radiation, ‘osmotic shock’, ferromagnetic vortex layer treatment, enzyme solution treatment, and 
antibiotics treatment. 
A comparative analysis of the extraction solvents used for the extraction of lipids allowed to conclude that the 
use of a mixture of polar and non-polar extraction solvents almost quadruples the recovery of lipids (3.95 
times as high) as compared to the extraction with non-polar solvent only. The optimum ratio of solvents of 
ethanol - petroleum ether 2:1 (vol.), and the temperature of 47÷50 °C provides the maximum degree of lipid 
recovery – 28 %. 
A mathematical model of the lipid extraction process has been developed and optimal conditions for the 
extraction have been determined. 

1. Introduction 
Lipid extraction from microalgae is a process that is characterised by high energy consumption. This 
significantly complicates the use of microalgae biomass as raw material for the production of a wide range of 
products on an industrial scale (Yang et al., 2014). Two types of processes of lipid extraction from microalgae 
biomass can be identified: extraction from wet biomass, wherein the extraction of the end product is difficult 
because of the cell culture fluid, which leads to a low recovery rate in the extraction process, and extraction of 
lipids from dry microalgae biomass, the drawback of which is high energy costs for drying the biomass. 
Thus, with the aim of reducing energy consumption and increasing lipid recovery, the methods of preliminary 
processing of microalgae biomass have been intensively studied (Table 1). 
From the literature review on the subject it can be concluded that no studies have been made to analyse the 
most effective ways of cell walls disruption and their influence on lipid recovery rate, as well as there is no 
consensus about what would be the best solvent for the extraction of lipids from biomass. In this regard, the 
aim of the present study was to determine the best conditions for maximum extraction of lipids from C. vulgaris 
microalgae biomass. 
To achieve this goal the following tasks were set and performed: 1) experimental determination of the most 
effective method of cells disruption of C. vulgaris IFR №С-111 strain, selection of the best extraction solvent, 
of solvent – biomass ratio, and temperature of extraction; 2) development of a mathematical model of the 
process of lipid transition from biomass to the solvent. 

                                

 
 

 

 
   

                                                  
DOI: 10.3303/CET1649030 

 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 
 

Please cite this article as: Dvoretsky D., Dvoretsky S., Temnov M., Akulinin E., Peshkova E., 2016, Enhanced lipid extraction from microalgae 
chlorella vulgaris biomass: experiments, modelling, optimization, Chemical Engineering Transactions, 49, 175-180  DOI: 10.3303/CET1649030

175



Table 1:  Literature review  

Study Biomass type Best disruption method Solvent 
Lipid 

recovery, 
% 

Araujo et al. 
(2012) 

C. vulgaris 
dry biomass  

ultrasound(40 kHz) 
Chloroform – 
methanol: 1:2 

(vol.) 
52.0 

Prommuak et 
al. (2011) 

C. vulgaris lyophilised 
biomass 

ultrasound(40 kHz), microwave 
radiation (300 W) 

Chloroform – 
methanol 
1:2 (vol.) 

38.9 

Zuorro et al.  
(2015)  

Nannochloropsis sр. 
lyophilised biomass 

Enzyme solution 
(galactomannanase, 1,4 β-

cellobiosidase and β-glucosidase)

n-hexane -  
2-propanol 
3:2 (vol.) 

37.3 

Concas et al. 
(2015)  

C. vulgaris wet biomass 
Fenton reaction: 0.5 mole/L Н2О2 

and 0.024 mole/L FeSO4 , 
treatment time up to 3 min. 

Ethanol – 
hexane mixture 

17.4 

Cho et al. 
(2013)  

C. vulgaris biomass of 
99 % moisture content 

Cellulase at рН=4.8, T= 50 °С, 
P=72 h 

Chloroform – 
methanol 
2:1 (vol.) 

10.0 

Lee et al. 
(2010)  

C. vulgaris dry biomass 
mixed with distilled water 

Autoclave treatment (125 °С at 
1.5 МPa for 5 min.), microwave 
radiation (2450 МHz for 5 min.) 

Chloroform – 
methanol 
1:1 (vol.) 

10.0 

2. Methods and materials 
2.1 Cultivation and concentration of biomass  

C. vulgaris IFR №С-111 strain was cultivated in the photobioreactor of 2 L volume, with the use of Tamiya 
OPTIMUM medium, at 30 °С and the illuminance level of 14 kLx for 8 days, before reaching the stationary 
phase of growth. After that, stress conditions (nitrogen deficit) were created for a period of 6÷7 days 
(Dvoretsky et al., 2015).  

The biomass was concentrated to a moisture content of 95÷98 % using a centrifuge with rotation speed 
3000 min-1 for 5 minutes. 

2.2 Cell walls breakage 

Cell walls of C. vulgaris microalgae were broken using the following disruption methods: 1) treatment with 
enzyme solution of CelloLux A and Protosubtilin g3x in 12 mg/mL – 4 mg/mL ratio and exposure time of 10 
min. at 55 °С; 2) treatment with amoxicillin solution 0.5 % (mass.) strength; 3) microwave radiation (power 700 
W, radiation frequency 280 МHz, treatment time 30 sec.); 4) ferromagnetic vortex layer treatment in 
electromagnetic field (FVLT) (m (ferromagnetic particles) = 3.85 g, treatment time 15 sec., value of magnetic 
induction of the rotating electromagnetic field - 0.13 T, the speed of rotation of the field - 30 s–1, magnetic 
moment 8.635·10-5 А·m2, rotational inertia 0.28·10-8 kg·m2, magnetic field intensity 398.01 А/m, size of 
ferromagnetic particles l = 12 mm, d = 1 mm); 5) ‘osmotic shock' (sodium chloride solution or sucrose solution 
is added to 15 % (mass.) biomass paste, and after 24 h the mixture is diluted in distilled water in 1:20 ratio). 
The determination of the number of intact cells before and after exposure was carried out by direct counting in 
the Goryaev chamber; the number of cells which lost viability, but retained their shape was counted by adding 
methylene blue dye to the biomass and directly counting stained cells in the Goryaev chamber. The number of 
disrupted cells was the difference in the number of cells before and after exposure. 

2.3 Lipid extraction 

Extraction of lipids from microalgae biomass with disrupted cell walls was carried out in a container with a 
magnetic stirrer (rotation speed 400 min

-1). Estimation of lipids extracted from biomass was done by Zoellner 
and Kirsch method of determination of total lipids (Zoellner and Kirsch, 1962). 
Distillation of the solvent was carried out using a rotary evaporator IR-1 M3 at a temperature of distillation 
85 °С and the speed of rotation of the flask 65 min-1.  

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3. Experimental research into the process of microalgae cell disruption and lipid extraction 
For the purpose of selecting an extraction solvent which allows extracting a maximum amount of intracellular 
lipids from C. vulgaris microalgae biomass, an experiment was conducted with the use of non-polar solvents 
(petroleum solvent C2 80/120, petroleum ether) and polar solvents (ethanol and isopropanol), and mixtures of 
ethanol and petroleum ether in the ratio 2:1 (vol.) and 1:1 (vol.) as extraction solvents. The results of the 
experiment are presented in Figure 1. These results allow to conclude that the largest lipid recovery 14.9 % of 
dry matter of biomass is observed when using a mixture of ethanol – petroleum ether 2:1 (vol.) as a solvent. 
This result can be explained by the fact that some neutral lipids are located in the cytoplasm not only in the 
form of lipid globules, but also as complexes with polar lipids. These complexes are attracted by hydrogen 
bonds to the proteins of the cell membrane. Van der Waals forces arising between non-polar organic solvent 
and the neutral lipids, which are composed of protein-lipid complexes, are not sufficient to destroy the 
attraction between lipids and proteins. On the other hand, a polar organic solvent (such as ethanol, 
isopropanol, etc.) is capable of disrupting the lipid-protein associations by forming hydrogen bonds with the 
polar lipids in the complex (Kates, 1986). However, along with the neutral lipids which are present in the cells 
in the form of globules and are included in membrane-associated complexes, polar lipids (phospholipids and 
glycolipids) are extracted as well. 
In order to determine an optimal biomass and extraction solvent ratio for maximum extraction of intracellular 
lipids from the biomass of C. vulgaris, an experiment was conducted with different ratios R of biomass (g) with 
a residual moisture content of 5 % and a mixture of solvents (ml) (ethanol – petroleum ether in 2:1 (vol.) ratio). 
The results of the experiment are presented in Figure 2. It can be concluded that the highest lipid recovery 
rate of 28 % of dry matter of biomass in the extraction was observed when the R ratio of the mixture was 1 (g) 
of biomass to 200 (ml) of a mixture of solvents. This result can be explained by the fact that a greater amount 
of solvent allows forming a greater number of Van der Waals interactions (non-polar solvent) and hydrogen 
bonds (polar solvent) with polar and non-polar lipids; consequently, the formation of more lipid-solvent 
complexes makes it possible to extract more lipids. Further increase in R leads to a small increment in the 
amount of the extracted lipids (up to 31 %), but it raises the cost of separation of the solvent by ≈ 8÷10 %. 

 
 

Figure 1: Dependence of lipid recovery on the type of 
extraction solvent 

Figure 2: Dependence of lipid recovery on extraction 
solvent and biomass ratio R 

One more experiment was set up to determine extraction temperature which allows extracting a maximum 
amount of lipids from C. vulgaris microalgae biomass. Lipids were extracted with a mixture of ethanol – 
petroleum ether in 2:1 (vol.) ratio, biomass – extraction solvent ratio R was 1 (g) : 100 (mL), and temperature 
range 25÷67 °С. The results of the experiment are presented in Figure 3. The largest lipid recovery rate of 
26 % of the dry matter of biomass was observed when the extraction temperature was 47 °C, which can be 
explained by the fact that when the temperature rises above 47 °C, the disruption of heat-labile components of 
the cell occurs, which leads to a decrease in recovery rate. 
With the aim of selecting the best method of breaking cell walls of C. vulgaris IFR №С-111 microalgae strains, 
an experiment was performed with the microalgae paste of 98 % moisture content. A cell wall in mature C. 
vulgaris cells has two layers (Burczyk and Hesse, 1981): the first layer is a three layer membrane, which 
consists of sporopollenin, the second layer consists of mannose and chitin. Such strong cell walls resulted in 
the fact that, after exposure to a disrupting influence, one part of the cells remained intact (Figure 4, sector A), 
another part of cells lost their viability but retained their shape and were permeable to substances (solvent or 
dye) from the external environment (Figure 4, sector B), and the third part of the cells were disrupted (Figure 

177



4, sector C). The results of experiments on the determination of the number of disrupted cells, damaged cells 
that preserved their structure, and intact cells are presented in Table 2. 

  

Figure 3. Dependence of lipid recovery on extraction 
temperature 

Figure 4: Microscopy of C. vulgaris cells after 
exposure to a disrupting influence 

Based on these measurements, the minimal number of cells remained intact when the biomass was treated 
with microwave radiation (Table 2), therefore, we can conclude that this is the most effective method of 
disrupting cell walls of C. vulgaris. This is further confirmed by the extraction of lipids from the samples of 
C. vulgaris biomass with cells that have been submitted to different methods of disruption (Table 3). 

Table 2:  Cell ratio after disruption 

Method of disruption Intact cells, % 
Non-viable cells that retained 

their shape, % 
Disrupted cells, % 

Antibiotic 88.6 5.4 6.0 
Enzymes 81.0 10.0 9.0 

Microwave radiation  7.7 43.8 48.5 
FVLT  79.0 12.0 9.0 

Sodium chloride solution 76.1 17.9 6.0 
Sucrose solution  85.5 9.5 5.0 

Table 3:  Lipid extraction depending on a method of cell disruption 

Method of disruption 
Lipid recovery, %  

Chl. vulgaris  IFR № С-111 
Antibiotic 10.0 
Enzymes 9.0 

Microwave radiation  15.0 
FVLT  15.0 

‘Osmotic shock’  7.0 

In order to determine the integrated impact of two methods of disruption on a cell wall during lipid extraction 
from C. vulgaris biomass with 90 % moisture content, an experiment was conducted according to the scheme 
presented in Table 4. The highest yield of total lipids (22.9 %) is observed when C. vulgaris cell walls are 
broken by integrated effects of 0.5 % antibiotic solution and microwave radiation, and lipids are extracted by 
petroleum ether and ethanol 1:2 (vol.) solvent mixture. 

4. Mathematical modelling of the process of lipid extraction from C. vulgaris biomass  
The modelling object is the extraction of lipids from C. vulgaris biomass, which contains cells of three types 
(intact, cells that retained the shape but are permeable to the solvent, disrupted, see Figure 4). 
Based on the analysis of experimental data it can be concluded that when building a mathematical models the 
following can be assumed: 1) biomass is a paste with 95 % moisture content; 2) the extractor allows for a 
perfect mixing; 3) all non-disrupted cells of the biomass have a radius r ≈ 3•10-6 m, surface area S; the cells 
that lost viability, but retained the shape have radius r, the surface area (S-Sh), where Sh is the area of the 
holes in the walls of cells (resulting from disruption), and lipid complexes have equivalent diameter 

178



de = 4•10
-9 m; 4) 100 % of lipids is extracted from the disrupted cells, 90 % of lipids is extracted from non-

viable cells (I = 0.9 is a coefficient of incomplete extraction of lipids from the cells which lost their viability, 
while preserving the shape), 70 % of lipids - from non-disrupted cells (J = 0.7 is a coefficient of incomplete 
extraction of lipids from intact cells); 5) wall thickness of all biomass cells is δ  = 10-7 m. 

Table 4:  Lipid extraction under the integrated disruption of biomass cells  

Method C. vulgaris IFR № С-111 
NaCl ‘osmotic shock’ + + - - - - 

Sucrose ‘osmotic shock’ - - + + - - 
Antibiotic - - - - + + 

FVLT  + - + - + - 
Microwave radiation - + - + - + 

Lipid recovery, % 19.6 20.1 15.3 17.7 17.9 22.9 

The extraction of lipids from the cells (intact, disrupted, and retaining its shape, but permeable to the solvent) 
can be described by mass transfer equation:  

),( * CCFK
dt
dC

V −⋅⋅=⋅  (1) 

where V is the extractor volume, m3; C* is the limiting concentration of lipids in the liquid phase (a mixture of 
biomass and solvent), mole/m3; C is the current concentration of lipids in the liquid phase, mole/m3 (a mixture 
of biomass and solvent), K is mass transfer coefficient, m/s; F is the surface area of contact of phases, m2. 
Depending on the type of cells in the biomass, the terms of Eq(1) are calculated as follows: 

1) for intact cells: 
Z

NPX
C

+
⋅⋅

=
1

* , 

( )βδ /12
1

int +





+






 ⋅⋅

=

D
D

n
r

K , where Х is an accumulated amount of 

biomass, Р is concentration of lipids, N is a share of intact cells,  Z is an amount of solvent added, 2r is cell 
diameter, m,  n is a coefficient; Dint is an internal diffusion coefficient, m

2/s; D is a coefficient of diffusion 
through a cell wall, m2/s; δ  is thickness of a cell wall, m; and β  is mass transfer coefficient, m/s. 

2) for non-viable cells which retained their shape: 
Z

RNPX
C

+
+−⋅⋅

=
1

))(1(* , 
( )β/12

1

int +







⋅⋅
=

D
n
r

K , where R 

is an amount of disrupted cells. 

3) for disrupted cells: Z
NPX

C
+

⋅⋅
=

1
* , where the mass transfer coefficient is determined by convection 

component β=K . 
The surface area of phase contact F were was determined based on the equivalent diameter of the molecules 
of the protein-lipid complex de, taking into account the number of free (unbound by solvent) lipid molecules: 

VNCCdF ae ⋅⋅−⋅⋅= )(
*2π , where Na is Avogadro's number. 

The equations of the model were solved by the Runge-Kutta fourth order method in the Matlab software. The 
adequacy was checked by comparing calculated and experimental values obtained under the following 
experimental conditions: X·P = 2.32 mole/m3; t = 30 °C; w = 2 m/s; N = 0.077; R = 0.485, a mixture of 
solvents: ethanol - petroleum ether 2:1 (vol.), R = 1:200 (Figure 5). The maximum mismatch was 10 %. From 
Figure 5 it follows that the implementation of the extraction for longer than 150 minutes is impractical since the 
bulk of the lipids is already extracted. 

 Figure 5: Extraction of lipids from biomass 
0 50 100 150 200 250 300

0

0.05

0.1

0.15

0.2

0.25

0.3

0.35

Extraction time, min

L
ip

id
s 

co
n

ce
n
tr

a
tio

n
, 

m
g
/m

l

 

 

exp
mod

179



5. Conclusions 
The conducted research has shown that the integrated application of antibiotic solution and microwave 
radiation to C. vulgaris biomass (95 % moisture content) yields the largest lipid recovery rate. The temperature 
of the biomass during the treatment process must not exceed 50 °C. It has been established that to extract the 
maximum total lipids a mixture of polar (ethanol) and nonpolar (petroleum ether) solvents in the ratio 2:1 (vol.) 
should be used. The ratio of the amount of dry biomass (g) to the amount of the mixture of solvents (ml) 
should be 1:100÷1:200, and extraction temperature – 45÷50 °C. It was experimentally determined that the 
extraction time during which the major part of lipids is extracted is ≈150 minutes. The mathematical model of 
the process of lipid transition from biomass to solvent was developed. 

Acknowledgments 

The work was commissioned and carried out with financial support of the Ministry of Education and Science of 
the Russian Federation. 

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