Professional Documents
Culture Documents
PROJECT REPORT
ON
A PROJECT REPORT
Submitted in partial fulfillment of the
Requirements for the award of the degree of
Master of Science
In
Department Of Biotechnology
By
NIRAV J GHANTALA
SURAT
2012
CERTIFICATE
ACKNOWLEDGEMENT
I thank the almighty whose blessings have enabled me to accomplish my dissertation work
successfully.
It is my pride and privilege to express my sincere thanks and deep sense of gratitude to Priya
Bande, Department of Biotechnology and Environmental Sciences, MITCON, pune for her
valuable advice, splendid supervision and constant patience through which this work was
able to take the shape in which it has been presented. It was her valuable discussions and
endless endeavors through which I have gained a lot. Her constant encouragement and
confidence-imbibing attitude has always been a moral support for me.
My sincere thanks to Dr.Chandrashekhar kulkarni, Head Department of Biotechnology and
Environmental Sciences, for his immense concern throughout the project work.
I also wish to thank all my friends, for providing the mandatory scholastic inputs during my
course venture.
Finally, I wish to extend a warm thanks to everybody involved directly or indirectly with my
work.
The whole credit of my achievements goes to my parents and my brother who were always
there for me in my difficulties. It was their unshakable faith in me that has always helped me
to proceed further.
DECLARATION
I hereby declared that the work presented in the Project entitled has been carried out by
GHANTALA NIRAV J. under the guidance of Priya Bande, Project Guide, at MITCON, Pune.
The entitled Work is original and no part of this work is either published or submitted in any
university for the award of any degree or diploma.
Date:
Place: Pune
S.NO. CONTENTS
PAGE.NO
1. Introduction
22
3.Observation Tables
29
4. Results
36
5. conclusion
41
6.References
41
7.Appendix
43
Abstract
1.INTRODUCTION
6
1.1General Introduction
Production of SCP by mass culture of microorganisms is yet to take momentum at industrial
scale and deserve much attention to solve the problem of starvation in the coming decades.
The criteria for microorganisms to be used as food or feed include 1.the organism must be
genetically stable, non toxic and grow rapidly on a simple non specific medium.2. it should
have high nutritional or vitamin content and should be edible to human and other animals.
The organisms should also utilize the energy source without producing any side effects and
any undesirable effects. 3. it should be easy to separate the cells from the medium and the
product must have good quality and composition. Among the various groups of
microorganisms used to produce SCP, yeasts are perhaps the most important groups because
yeasts produce many bioactive substances such as proteins, amino acids, vitamins,
polysaccharides, fatty acids, phospholipids, polyamines, astaxanthins, -carotenoids,
trehalose, glutathione, superoxide dismutase, chitinase, amylase, phytase, protease, killer
toxin etc. which have been receiving much attention for many decades. The main nutritional
contribution in either human food or animal feed is its high protein content. Because of high
protein and fat content, the contribution of carbohydrates to the nutritional value of SCP is
not of prime importance. But a major constraint for yeast as SCP is the thick cell wall which
is difficult to digest leading to poor protein bioavailability.
Agricultural activities and food industry generate considerable quantities of wastes which are
rich in organic matter and could constitute new materials for value added products. A
growing concern for the acute food shortages for the worlds expanding population has led to
the exploitation of non-conventional food sources as potential alternatives. Among these, the
single cell organisms probably present the best chances for the development of unique
independence of agricultural crop based food supply.
Single cell protein is a biomass based on protein extract derived from microorganism.Single
cell protein offers numerous advantages for the productions of proteins because of its high
productivity,low cost media,less effort and product with added
nutritional market
value(pandey et al.,1992). The single cell protein is a dehydrated cell consisting of mixture of
proteins, lipids,carbohydrates, nucleic acids, inorganic compounds and a variety of other non protein
nitrogenous compounds such as vitamins. Agricultural wastes are useful substrate for production of
microbial protein, but must meet the following criteria; it should be non toxic, abundant, totally
regenerable,non-exotic, cheap and able to support rapid growth and multiplication of the organisms
resulting in high quality biomass.
There have been studies as well as efforts to improve the protein quantity and quality of the
finished food products by augmenting protein-rich cheaper ingredients in food formulations
(Nasir and Butt, 2011;Hussain et al., 2007). Although animal proteins are considered to be
best quality proteins (Saima et al., 2008), however microbial protein also known as single
cell protein grown on agricultural wastes is one of the important optional proteins because of
higher protein content and very short growth cycle of microorganisms,thereby, leading to
rapid biomass production (Bekatorou et al., 2006) Moreover, microbes are also able to grow
on cheap nutrient sources resulting in economical,potentially supplemental protein biomass
for balanced nutrition.
The UN work for the servey of food consumption of worldwide.It recently reported that over
1 billion people currently do not have access to adequate amounts of food and that number
could climb even higher in the near future if current drought conditions persist. Based on UN
research, it was estimated a decrease in agricultural production of 20-40% if drought
conditions continue and concluded that 2009 could be the beginning of a record-breaking
humanitarian crisis throughout much of the world.The demand for protein as food is
expanded for malnourished human populations. Consequently,the cost of protein secondary
use as food for livestock has also risen. Increasingly there was always a stimulus needed to
introduce an additional and or complementary source of animal feed microorganisms that are
considered for food or feed use including algae, bacteria, yeasts, molds, and higher fungi. The
dried cells of these organisms are collectively referred to as single cell protein. Different
types of microorganisms have been recommended for human consumption, including yeast,
molds and algae. But as of now only yeast have been used as food to any extent and then
under unusual conditions. During Second World War when there were shortages in proteins
and vitamins in the diet, the Germans produced yeast and mold Geotrichum candidum in
some quantity for food. Research on single cell protein has been stimulated by food crisis or food
shortages that will occur if the worlds populations are not controlled. Scientists believe that use of
microbial fermentations and the development of an industry to produce and supply single cell proteins
from agricultural waste are insufficient.
The present study was focused on yeast single cell protein rather than bacterial, fungal and algal
single cell protein. Algal single cell protein have limitations such as the need for warm temperatures
and plenty of sun light in addition to carbon dioxide, and also that the algal cell wall is indigestible.
Bacteria are capable of growth on a wide variety of substrates, have a short generation time and are
high protein content. Their use is somewhat limited by poor public acceptance of bacteria as food,
small size and difficulty of harvesting and high content of nucleic acid on a dried weight basis. Yeasts
are probably the most widely accepted and used microorganisms for single cell protein. These include
strains of Candida utilis, C. arborea, C. pulcherrima and Saccharomyces cerevisiae.Pichia stipitis is
also used for SCP production in the present study. In recent years increasing attention has been
given to the conversion of food processing wastes into valuable by-products such as the
production of yeast protein from potato (Skogman 1976) and confectionery effluents (Forage
1978). The recovery of such by-products can significantly reduce the costs of waste disposal.
10
with conventional sources of protein (soybeans or meat) are well known.A number of
agricultural and agro industrial waste products have been used for the production of SCP and
other metabolites, including orange waste, mango waste, cotton salks, kinnowmandarinwaste, barley straw, corn cops, rice straw, cornstraw, onion juice and sugar cane
bagasse (Nigam et al., 2000), cassava starch (Tipparat et al., 1995), wheat straw (Abou
Hamed, 1993), banana waste (Saquido et al., 1981), capsicum powder (Zhao et al., 2010) and
coconut water (Smith and Bull, 1976). The usage of such wastes as a sole carbon and
nitrogen source for the production of SCP by microorganisms could be simply attributed to
their presence in nature on large scale and their cheap cost.
12
affiliation of the yeast species and on the culture media used. The high percentage of
polyunsaturated fatty acids (PUFAs) found in Patagonian yeasts, in comparison to other
yeasts, is indicative of their cold-adapted metabolism.
Yeast proteins are easily digestible compared to those from bacteria. Chemical analysis of
microorganisms tested for SCP reveal that they are comparable in amino acid content to the
plant and animal sources with the exception of sulphur amino acid methionine which is low
in some SCP sources, especially yeasts. However, this can be alleviated by culturing yeasts
on molasses (Bhalla et al., 1999). The only species of yeast fully acceptable as food for
humans is S. cerevisiae (bakers and brewers yeast) (Bekatorou et al., 2006).
The majority of the SCP are either deficient in one or more amino acids or they suffer from
an amino acid imbalance (Tacon and Jackson, 1985; Kiessling and Askbrandt, 1993). The
supplementation of yeast-based diets with the deficient amino acids was shown to have
beneficial effects on fish growth (Nose, 1974; Spinelli et al., 1979; Murray andMarchant
1986).
Another concern with SCP is their high concentration in nucleic acids, ranging from 5 % to
12 % in yeast and 8 % to 16 % in bacteria (Schulz and Oslage, 1976). In rapidly proliferating
microbial cells, RNA forms the bulk of nucleic acids. The RNA content of yeast cells is
known to be dependent on the culture conditions and C/N ratios. The marine yeasts with high
levels of nucleic acids could be used as a feed to marine animals because some of them can
produce uricase which convert uric acid, the toxic intermediate of nucleic acid catabolism
into the non-toxic allantoin. The nutritional value of the yeast depends also on the
concentrations of other micronutrients such as sterols, vitamins and minerals. Yeasts have
usually high concentrations of sterols (typically 1-10 % of total lipids) which are required for
growth and survival of molluscs (Brown et al., 1996).
13
14
15
In anaerobic conditions, glucose is slowly utilized to produce the energy required just to keep the
yeast cells alive. This process is called fermentation, in which the sugars are not completely
oxidized yielding CO2 and ethanol (Scragg, 1991; Bekatorou et al., 2006) as final product. When
the yeast cell is exposed to high glucose concentration, catabolite repression occurs, during which
gene expression and synthesis of respiratory enzymes are repressed, and fermentation prevails
over respiration(Rincon et al.,2001: Bekatorou et al.,2006).
In industrial practice, catabolite repression (repression of gluconeogenesis, the glyoxylate cycle,
respiration and the uptake of less preferred carbohydrates) by glucose and sucrose, also known as
Crabtree effect, may lead to several problems, such as incomplete fermentation, development of
off flavors and undesirable by products as well as decreased biomass and yeast vitality
(Verstrepen et al., 2004; Bekatorou et al., 2006).
Industrial production of Saccharomyces cerevisiae is therefore, performed in aerobic, sugar
limited fed-batch cultures (Van Hoek et al., 1998; Mickiewicz and Borowiak, 2005).
16
When the yeast cell is exposed to high glucose concentration, catabolite repression occurs, during
which gene expression and synthesis of respiratory enzymes are repressed, and fermentation
prevails over respiration(Rincon et al.,2001: Bekatorou et al.,2006).
In industrial practice, catabolite repression (repression of gluconeogenesis, the glyoxylate cycle,
respiration and the uptake of less preferred carbohydrates) by glucose and sucrose, also known as
Crabtree effect, may lead to several problems, such as incomplete fermentation, development of
off flavors and undesirable by products as well as decreased biomass and yeast vitality
(Verstrepen et al., 2004; Bekatorou et al., 2006).
Industrial production of Saccharomyces cerevisiae is therefore, performed in aerobic, sugar
limited fed-batch cultures (Van Hoek et al., 1998; Mickiewicz and Borowiak, 2005).
17
1.3.2 Aeration
Highly aerobic culture conditions are used in the production of yeast specifically
bakers yeast to maximize cell growth (Campelo and Belo, 2004). The modern
technique of bakers yeast production is based on applying the principle of the Pasteur
reaction at the limit value of its aeration. Pasteur defined fermentation as life without
air. Its biochemistry involves the breakdown of carbohydrates only to the stage of
ethanol.
Under aerobic conditions, however, maximum growth occurs and the efficiency of
utilization of carbohydrate increases as respiration and the breakdown of the
carbohydrate to carbon dioxide and water becomes complete (Cook, 1958).
Generally oxygen has the following basic functions (Prescott and Dunn, 1959).
1. Inhibits fermentation
2. Increases respiration
3. Agitation of the medium
4. Removal of toxic end products
5. Stimulation of vegetative growth
18
Oxygen is used in the synthesis of unsaturated fatty acids and sterols which form the cell
membrane. These molecules are important for both growth and fermentation and serve as a means
for storing oxygen within the cell. They are also necessary for increasing cell mass (growth)
involving the over all uptake of nutrients and determining alcohol tolerance. Oxygen stimulates
the synthesis of molecules necessary for yeast to metabolize and take up maltose and other sugars
1.3.3. Temperature
The temperature most favorable to the growth of bakers yeast varies from strain to strain.
Optimum temperature is usually between 25 0C-350C. The maximum survival temperature is
370C (Cook, 1958). Propagation at low temperature, the rate of growth is slower and gives a
decreased yield of yeast. Yeast grown in low temperature is less stable when stored and
transported as a pressed cake and the dry matter of a yeast cake of standard consistency becomes
progressively less at low temperature, i.e., it affects the relationship between intracellular and
extra cellular water content.
1.3.4 pH
Yeasts grow well at acidic pH (acidophilic organisms). For industrial propagation low pH is
helpful in restricting the development of many bacterial contaminations; however, the color of the
yeast may be affected at low pH. The pH of the media is commonly adjusted by the addition of
H2SO4, NH3, Na2CO3 or NaHCO3 (Prescott and Dunn, 1959) to the substrate.
19
carbon (C)
Hydrogen ( H)
Oxygen ( O)
Nitrogen (N)
Total ash
Phosphate ( P2O5)
45.0-49.0
5.0- 7.0
30.0 -35.0
7.1 -10.8
4.7- 10.5
1.9- 5.5
Potash ( K2O)
1.4- 4.3
Calcium (CaO)
Magnesium ( MgO )
Aluminum ( as Al2O3)
0.005 0.2
0.1 0.7
0.002 0.02
Sulphate ( as SO4)
0.01- 0.05
These four elements are present on the yeast in the form of carbohydrates (glycogen,
cellulose, and yeast mannan), protein and lipids (true fats, lecithin, and sterols). Yeasts also
contain high amount of vitamin B complex, nucleic acids and organic bases (pyramidine and
purine bases). The inorganic substances may constitute up 6 to 8 % of the yeast dry matter
(White,1954;Roman,1957) Table 4 gives the quantities of some substances present in yeast
dry matter (White, 1954).
Ash
Normally 6 -8
20
Glycogen
Fat soluble fraction(true fats, sterols. lipids
Yeast gum (mannan )
Cellulose ( yeast )
Proteins and organic nitrogenous bases
1 -30
1 -2. 2
Up to 4
Up to 5
44 47
REVIEW OF LITERATURE
The work carried out on Comparative assessment of various agro-industrial wastes for
Saccharomyces cerevisiae biomass production and its quality evaluation as Single cell
protein(U. Bacha, M. Nasir, A. Khalique, A. A. Anjum* and M. A. Jabbar in 2011)
This study was planned to assess the feasibility of using agro-industrial wastes for
Saccharomyces cerevisiae production and to evaluate protein quality of produced single cell
protein (SCP) biomass. Potato peels contained significantly highest dry matter and
carbohydrate content as compared to other wastes. Significantly higher SCP biomass was
produced using potato peels followed by carrot peels. On the basis of higher SCP biomass
production, potato peels were selected for further biomass production. The SCP biomass
contained 49.291.126% crude protein which was non-significant (P=0.1710) compared to
commercially available Saccharomyces cerevisiae. The parameters for in-vivo protein quality
assay in Sprague Dawley rats were; 93.68% true digestibility, 67.02% net protein utilization,
70.56% biological value, 4.55net protein ration, and 2.75 protein efficiency ratio, which are
higher in comparison to most of cereal proteins. The present exploration depicted that
Saccharomyces cerevisiae can be efficiently produced utilizing wastes and the produced
biomass can potentially be used as protein source in various food formulations.
The work carried out on Production of Single cell protein from Pineapple waste using
yeast(Dharumadurai DHANASEKARAN1*, Subramaniyan LAWANYA, Subhasish SAHA1,
Nooruddin THAJUDDIN 1, Annamalai PANNEERSELVAM2)
21
In this work pineapple waste was used as sole carbon source in five concentrations for
preparation of fermentation media on which two strains of yeasts, Saccharomyces cerevisiae
and Candida tropicalis were grown. The increased concentration of pineapple hydrolysate
enhanced the biomass yield and the protein formation within the yeast cells. Lower carbon
utilization by the two yeast strains occurred in the wastecontaining media, as compared to
control, increasing the economic value of the waste obtained after 7-day fermentation.
(a) GLASSWARE
Petri dishes,
Glass slides,
Glass beakers,
Cover slips,
Media bottles,
Conical flasks,
Pipette,
Test tubes,
(b )REAGENTS REQUIRED
Alcohol,
Distilled water,
Ethanol
Concentric sulfuric acid
(c)EQUIPMENTS REQUIRED
22
Ph meter
Inoculating loops,
Weighing machine,
Incubator,
Autoclave(Meta instrument,Mumbai),
Refrigerator,
Laminar air flow,(Microfilt)
Microscope,
Measuring cylinder
Spectrophotometer
Vortex machine
Centrifuge(Remi)
Waterbath
market.Pineapple waste and Orange peels were cut into slices in order to hydrolysis.Put this
slices in oven at 135 C for 24 hours For the moisture content to know.
2.2MICROORGANISM
The yeast culture such as Saccharomyces cerevisiae ,Candida tropicalis and pichia stipitis were
obtained by using isolation. The cultures were maintained on slant of yeastpeptone dextrose
medium(Yeast extract 10g, Dextrose 20g, Peptone 20g, Agar 20g, pH = 6.0,Distilled water 1000ml)
and stored at 4oC.Aspergillus niger is also used in this study.
The yeasts culture was used in the experiments because of its ability to ferment sugar. The
cultures of yeasts were isolated from soil by pour plate method. Dry powdered yeast (Instant
Yeast, Levure Instantane) was also used. The samples were streaked on YPD-agar medium
23
composition yeast extract (3.0g/L); peptone (10g/L); dextrose (20g/L); agar-agar (15g/L)
(YPG-agar) and incubated at 30C for 24h.. The best culture was selected for further studies.
Selected cultures were stored at 4C
2.3 METHODS
2.3.1 ISOLATION OF Aspergillus niger
1. Soil samples were collected from agriculture college campus,pune.
2. 1 g of each soil sample was individually suspended in 1 mL of sterile distilled water
3. Serially diluted to 103 fold
4. And plated on potato dextrose agar (PDA) plates containing kanamycin to a final
concentration of 106.
5. The plates were incubated at 30 C for 3 days in an environmental chamber under
controlled conditions.
6.Single colony of fungus was isolated and transferred repeatedly to a new PDA plate
until pure cultures were obtained. These were grown on PDA slants as above and
stored at 4C.
were the colonies, which are light yellow in colour; round in shape, smooth,
slightly convex i.e. bulged in the Petri plates.
2.4 FERMENTATION
2.4.1 PROCEDURE
1.Five media, other than control, were prepared.
2.Control consisting of the basal media (D-glucose-10.0g; (NH2)2SO4 5.0g ; KH2PO4
1.0g ; MgSo4, 7H2O 0.5g ; NaCl 0.1g ; CaCl2 0.1g ; Distilled water 1000 ml ; pH
5.5)with glucose
3.Other media were not free from glucoses but supplied with 1 to 5% pineapple hydrolysate.
4.The medium were distributed in Erlenmeyer flasks and sterilized at 121oC for 15 minutes.
5.The Yeast strains were inoculated in the media and incubated at 28oC for 7 days.
6, The yeast cells were separated by washing from the fermented broth and analyzed
7.Other synthetic media also used for the Single cell protein production..
5.1 The moisture content of the sample is calculated using the following equation:
A=A-B/B x 100
Where:
%W = Percentage of moisture in the sample,
A = Weight of wet sample (grams), and
B = Weight of dry sample (grams)
5.2 Report the moisture content to the nearest tenth of one percent.
PROCEDURE
26
2. Hydrolyse by keeping it in a boiling water bath for three hours with 5 mL of 2.5 N HCl and
cool to room temperature.
3. Neutralise it with solid sodium carbonate until the effervescence ceases.
4. Make up the volume to 100 mL and centrifuge.
5. Collect the supernatant and take 0.5 and 1 mL aliquots for analysis.
6. Prepare the standards by taking 0, 0.2, 0.4, 0.6, 0.8 and 1 mL of the working standard.
0 serves as blank.
7. Make up the volume to 1 mL in all the tubes including the sample tubes by adding
distilled water.
8. Then add 4 mL of anthrone reagent.
9. Heat for eight minutes in a boiling water bath.
10. Cool rapidly and read the green to dark green colour at 630 nm.
11. Draw a standard graph by plotting concentration of the standard on the X-axis versus
absorbance on the Y-axis.
12. From the graph calculate the amount of carbohydrate present in the sample tube.
CALCULATION
Amount of carbohydrate present in 100 mg of the sample= mg of glucose
100
Volume of test sample
NOTE:
Cool the contents of all the tubes on ice before adding ice-cold anthrone reagent.
27
2. Add 100 L of each of the above to a separate test tube (or spectrophotometer tube if
using a Spec 20).
3. Add 5.0 mL of Coomassie Blue to each tube and mix by vortex, or inversion.
4. Adjust the spectrophotometer to a wavelength of 595 nm, and blank using the tube
which contains 0 BSA.
5. Wait 5 minutes and read each of the standards and each of the samples at 595 nm
wavelength.
6. Plot the absorbance of the standards vs. their concentration. Compute the extinction
coefficient and calculate the concentrations of the unknown samples.
3.OBSERVATION TABLE
1.BRADFORD METHOD
28
STANDARD
SR NO.
STD
DIST.WATER
COOMASIAE O.D
SOLUTION(ML
BRILLIANT
BLUE(ml)
BLANK
5.0
1.0
0.00
0.2
4.8
1.0
0.16
0.4
4.6
1.0
0.32
0.6
4.4
1.0
0.50
0.8
4.2
1.0
0.63
1.0
4.0
1.0
0.76
FOR SAMPLE(S.cerevisiae)
PINEAPPLE WASTE
1%
0.5
4.5
0.15
2%
0.5
4.5
0.27
3%
0.5
4.5
0.32
4%
0.5
4.5
0.58
5%
0.5
4.5
0.73
Candida tropicalis
1%
0.5
4.5
0.10
2%
0.5
4.5
0.23
3%
0.5
4.5
0.39
4%
0.5
4.5
0.55
5%
0.5
4.5
0.66
29
Pichia stipitis4.5
1%
0.5
4.5
0.08
2%
0.5
4.5
0.12
3%
0.5
4.5
0.33
4%
0.5
4.5
0.49
5%
0.5
4.5
0.53
1%
0.5
4.5
0.10
2%
0.5
4.5
0.12
3%
0.5
4.5
0.32
4%
0.5
4.5
0.48
5%
0.5
4.5
0.54
Aspergillus niger
1%
0.5
4.5
0.07
2%
0.5
4.5
0.12
3%
0.5
4.5
0.28
4%
0.5
4.5
0.41
5%
0.5
4.5
0.53
Candida tropicalis
1%
0.5
4.5
0.09
2%
0.5
4.5
0.13
30
3%
0.5
4.5
0.20
4%
0.5
4.5
0.38
5%
0.5
4.5
0.55
1%
0.5
4.5
0.06
2%
0.5
4.5
0.15
3%
0.5
4.5
0.22
4%
0.5
4.5
0.36
5%
0.5
4.5
0.44
1%
0.5
4.5
0.11
2%
0.5
4.5
0.17
3%
0.5
4.5
0.30
4%
0.5
4.5
0,43
5%
0.5
4.5
0,56
Pichia stipitis
Aspergillus niger
4%
0.5
4.5
0.39
C.t
4%
0.5
4.5
0.32
P.s
4%
0.5
4.5
0.31
A.n
4%
0.5
4.5
0.30
ORANGE PEEL
31
S.c
4%
0.5
4.5
0.38
C.t
4%
0.5
4.5
0.34
P.s
4%
0.5
4.5
0.27
A.n
4%
0.5
4.5
0.29
SR NO.
ALIGUOTES
DISTILLED
DNSA
(ml)
WATER(ml)
REAGENT
40%
O.D
Rochelle
salt
solution(
1.
2.
3.
4.
5.
6.
BLANK
0.2
0.4
0.6
0.8
1.0
2.0
1.8
1.6
1.4
1.2
1.0
3.0
3.0
3.0
3.0
3.0
3.0
ml)
1
1
1
1
1
1
0.00
0.09
0.25
0.38
0.50
0.62
PINEAPPLE WASTE
1%
0.13
2%
0.24
3%
0.31
4%
0.47
5%
0.56
0.09
Candida tropicalis
1%
32
2%
0.17
3%
0.27
4%
0.36
5%
0.44
Pichia stipitis
1%
0.10
2%
0.19
3%
0.28
4%
0.39
5%
0,.46
Aspergillus niger
1%
0.08
2%
0.16
3%
0.22
4%
0.32
5%
0.40
1
FOR ORANGE PEELS
Saccheromyces cerevisiae
1%
0.08
2%
0.17
33
3%
0.30
4%
0.42
5%
0.51
Can1dida tropicalis
1%
0.08
2%
0.13
3%
0.27
4%
0.36
5%
0.45
Pichia stipitis
1%
0.12
2%
0.22
3%
0.35
4%
0.42
5%
0.48
Aspergillus niger
1%
0.13
2%
0.20
34
3%
0.31
4%
0.40
5%
0.47
4%
0.23
C.t
4% 1
0.29
P.s
4%
0.36
A.n
4% 1
0.44
ORANGE PEEL
S.c
%
0.25
C.t
4% 1
0.27
P.s
4%
0.35
A.n
4% 1
0.42
3.ANTRONE METHOD
SR NO.
1.
2.
3.
4.
5.
6.
ALIGUOTES
DISTILLED
ANTHRONE
(ml)
BLANK
0.2
0.4
0.6
0.8
1.0
WATER(ml)
2.0
O.8
0.6
0.4
0.2
0.0
REAGENT
4.0
4.0
4.0
4.0
4.0
4.0
35
O.D
0.00
0.13
0.27
0.42
0.54
0.66
PINEAPPLE WASTE
Saccharomyces cerevisiae
1%
0.5
1.5
0.11
2%
0.5
1.5
0.24
3%
0.5
1.5
0.32
4%
0.5
1.5
0.45
5%
0.5
1.5
0.53
Candida tropicalis
1%
0.5
1.5
0.09
2%
0.5
1.5
0.20
3%
0.5
1.5
0.29
4%
0.5
1.5
0.42
5%
0.5
1.5
0.48
Pichia stipitis
1%
0.5
1.5
0.09
2%
0.5
1.5
0.22
3%
0.5
1.5
0.29
4%
0.5
1.5
0.43
5%
0.5
1.5
0.52
36
Aspergillus niger
1%
0.5
1.5
0.12
2%
0.5
1.5
0.26
3%
0.5
1.5
0.32
4%
0.5
1.5
0.43
5%
0.5
1.5
0.54
1%
0.5
1.5
0.07
2%
0.5
1.5
0.16
3%
0.5
1.5
0.30
4%
0.5
1.5
0.42
5%
0.5
1.5
0.51
Candida tropicalis
1%
0.5
1.5
0.06
2%
0.5
1.5
0.18
3%
0.5
1.5
0.26
4%
0.5
1.5
0.40
5%
0.5
1.5
0.52
1.5
0.09
Pichia stipitis
1%
0.5
37
2%
0.5
1.5
0.14
3%
0.5
1.5
0.26
4%
0.5
1.5
0.39
5%
0.5
1.5
0.50
Aspergillus niger
1%
0.5
1.5
0.10
2%
0.5
1.5
0.14
3%
0.5
1.5
0.27
4%
0.5
1.5
0.42
5%
0.5
1.5
0.50
4%
0.5
1.5
0.29
C.t
4%
0.5
1.5
0.31
P.s
4%
0.5
1.5
0.33
A.n
4%
0.5
1.5
0.42
1.5
0.26
ORANGE PEEL
S.c
%
0.5
38
C.t
4 % 0.5
1.5
0.28
P.s
4%
0.5
1.5
0.33
A.n
4 % 0.5
1.5
0.41
4.RESULT
4.1IDENTIFICATION OF FUNGI
The fungus isolated from soil was identified as Aspergillus niger by theire
morphological characteristics, cultural characterstics,Conidiospores were found
upright,simple,terminating in a globose or swelling bearing phialides at the apex and or
radiating from the entire surface,conidia was one celled,globose,variously colored in the
mass,catenulate,produced basipetally.
39
The S. cerevisiae recorded high protein content (186mg/100ml). The protein content
increased with increase in concentration of carbon source inthe medium. The maximum
protein content of S.cerevisiae was recorded on 7th day of the fermentation at 5%
concentration of pineapple waste followed by
C.tropicalis (168mg/100ml),pichia
ORANGE PEELS
The C.tropicalis recorded high protein content (140 mg/100ml). The protein content
increased with increase in concentration of carbon source inthe medium. The maximum
protein content of C.tropicalis was recorded on 7th day of the fermentation at 5%
concentration of pineapple waste followed by S.cerevisiae (134 mg/100ml),pichia stipites(112
mg/ml) and Aspergillus niger ( 140 mg/100ml)
40
PINEAPPLE WASTE
In general the reducing sugar content increased with the increase in the concentration of
carbon source in the yeast basal medium. The content of reducing sugar in the yeast was
reduced from 11.0mg/100 ml to 4.36 mg/100ml on 7th day of observation on fermentation
process. Among the four isolates used in the study S. cerevisiae recorded highest reducing sugar
(6.64mg/100ml) followed by C. tropicalis (5.91 mg/100ml).
ORANGE PEELS
The content of reducing sugar in the yeast was reduced from 9.45 mg/100 ml to 3.75
mg/100ml on 7th day of observation on fermentation process. Among the four isolates used
in the study S. cerevisiae recorded highest reducing sugar (5.70 mg/100ml) followed by C. tropicalis
(4.92 mg/100ml).
ORAGE PEEL
The total sugar estimate is highest in C.tropicalis (19.8 mg/100 ml )and S.cerevisiae (17.9
mg/100ml) and lowest in Pichia stipitisd(14.6 mg/100ml).
pineapple has rapidly promoted growth of yeast cells. Concerning protein content, the highest
protein content was recorded on the 3rd day of fermentation at 5% concentration and
thereafter decreased. The present findings are in agreement with the findings of Abou Hamed
(1993). The protein content increased as the concentration of wheat straw hydrolysate
increased, at the same time the protein content gradually decreased when the fermentation
period increased.
5.CONCLUSION
The bioconversion effect of pineapple waste into SCP was evaluated using yeast. The
increase in biomass contents were observed when there was increase in pineapple waste
concentration. The highest biomass content of S. cerevisiae and C. tropicalis was recorded on
7th day fermentation. The highest protein content of S.cerevisiae and C tropicalis was
recorded on the 7th day of fermentation at 5 % concentration. The highest reducing sugar
content of yeast was recorded on 3 rd day of fermentation at 5% concentration. The utilization
of reducing sugar was increased with the increase in the concentration of substrates. The
present findings reveals that pineapple waste can be used as effective alternate carbon source
for SCP production. Also the orang peels have the same effects on all the para meters.
6.REFERENCES
Argyro, B., Costas, P., Athanasios, A.K. (2006). Production of Food Grade Yeasts. Food
Technol. Biotechnol. 44, 407415.
Nigam, N.M. (2000). Cultivation of Candida langeronii in sugarcane bagasse hemi cellulose
hydrolysate for the production of single cell protein. W.J.Microbiol.and biotechnol. 16, 367372.
43
Tipparat, H., Kittikun, A.H. (1995). Optimization of single cell protein production from
cassava starch using Schwanniomyces castellii. W.J. Microbiol. & Biotechnol. 11, 607-609.
Abou Hamed, S.A.A. (1993). Bioconversion of wheat straw by yeast into single cell protein.
Egypt. J. Microbiol. 28(1), 1-9.
Saquido, P.M.A., Cayabyab, V.A ., Vyenco, F.R. (1981). Bioconversion of banana waste into
single cell protein. J. Applied Microbiol. &Biotechnol. 5(3), 321-326.
Zhao, G., Zhang, W., Zhang, G. (2010). Production of single cell protein using waste
capsicum powder produced during capsanthin extraction. Lett Appl Microbiol. 50. 187-91.
Smith, M.E., Bull, A.T. (1976). Protein and other compositional analysis of Saccharomyces
fragilis grown on coconut water waste. J. Applied Bacteriol. 41, 97-107.
AOAC. (1975).Official methods of Analysis, 16th edition, Association of official Analytical
chemists, Washington D.C.
Ranganna, S. (1978). Handbook of analysis and quality of fruit and vegetable products, Tata
McGraw Hill Publishing Co. Ltd, New Delhi
Sadhu, M.K., Chattopadhy, P.K. (2001). Introduction to fruit crops. Naya Prakash Publication,
Calcutta, 252.
Phaff, H.J., Miller, M.W., Mark, E.M. (1996). The life of yeasts. Harvard university press, Cambridge,
Massachrsetts. 186.
Fawcett, J.K., Scott, J.E. (1960). A rapid and precise method for determination of urea. J. Clin. Path.
13, 156.
Krishnaveni. S., Theymoli, B., Sadasivam, S. (1984). Estimation of reducing sugar by dinitrosalicylic
acid method. Food Chem. 15, 186.
Hedge, J.E., Hofreiter, B.T. (1962). Carbohydrate Chemistry 17 th Edition, Whistler RL and Be Miller,
J.N. Academic Press New York.
Karla, K.L., Grewal, H.S., Kahlon, S.S. (1989). Bioconversion of kinnowmandarin waste in to single
cell protein. J. Appl. Microbial Biotechnol. 5(3), 153-157.
Rashad, M.M., Moharib, S.A., Jwanny, E.W. (1990). Yeast conversion of mango waste or methanol to
SCP and other metabolites. Biol. Waste. 32(4), 277.
Prosser, J.I., Tough, A.J. (1991). Growth mechanism and growth kinetics of filamentous
microorganism. Critical Reviews in Biotechnol. 10(4), 253-274.
7.APPENDIX
44
MEDIA
1) POTATO DEXTROSE AGAR
Potato Infusion
300g
Dextrose
20g
Agar
20g
PH
3.5
Distilled water
1000ml
20g,
Peptone
20g,
Agar
20g,
pH
6.0
Distilled water
1000ml
3) basal media
D-glucose
10.0g;
(NH2)2SO4
5.0g
KH2PO4
1.0g
MgSo4, 7H2O
0.5g
NaCl
0.1g
CaCl2
0.1g
Distilled water
1000 ml
pH
5.5
REAGENTS REQUIRED
1.2.5 N HCl
45
2. Anthrone reagent:
Dissolve 200 mg anthrone in 100 mL of ice-cold 95% H2SO4. Prepare fresh before
use.
3. Standard glucose:
StockDissolve 100 mg in 100 mL water. Working standard of stock diluted to 100
mL with distilled water. Store refrigerated after adding drops of toluene.
4.Dinitrosalicylic Acid Reagent (DNS Reagent)
Dissolve by stirring 1 g dinitrosalicylic acid, 200 mg crystalline phenol and 50 mg sodium
sulphite in 100 mL 1% NaOH. Store at 4C. Since the reagent deteriorates due to sodium
sulphite, if long storage is required, sodium sulphite may be added at the time of use.
5.40% Rochelle salt solution (Potassium sodium tartrate).
6.Standard bovine serum albumin (BSA)(1 mg/ml)
7.Coomassie Brilliant Blue 1
8 0.15 M NaCl
Dissolve 0.877g sodium chloride in 1000 ml Distilled water
46