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UNIVERSITI KUALA LUMPUR MALAYSIAN INSTITUTE OF CHEMICAL AND BIOENGINEERING TECHNOLOGY
FERMENTATION TECHNOLOGY (CBB20203 )
MINI PROJECT
PRODUCTION OF LACTIC ACID (MATERIAL & PROCEDURE)
GROUP
: MOHD SALEHAN BIN HASSAN
55202210266
AHMAD SHAFIQ BIN AHMAD FUAD
55202210134
MOHAMAD NORAZWAN BIN BAHARIN
55202210381
QAIYYUM AZIZI BIN MOHD NOOR
55202210221
SECTION
: 3 BCB EX
LECTURER
: SHARIFAH SOPLAH BT. SYED ABDULLAH
MATERIAL: A) Bacteria:
y
Lactobacillus
sp.
B) Chemical:
y
Glucose.
y
Yeast
y
Ammonium
y
Manganese
y
Cor n
y
Distilled
y
y
extract. hydr ogen phosphate, (NH4)2HPO4
sulf ate,
MnSO4
steep liquor. water.
Natr ium hydr oxide, NaOH. Hydr ochlor ic acid, HCL.
C) Apparatus:
y
2 L Bioreactor
y
Incubator
y
50 ml
y
250 ml Er lenmeyer flask
y
Loo p
y
1l
y
1L Measur ing
shaker
Er lenmeyer flask
Beaker cylinder
METHODS: A) Inoculum:
y
Prepare 30 g/L of glucose, 10 g/L of yeast extract, 2g/L of (NH4)2HPO4, and 0.1 g/L of MnSO4 in 1L of distilled water.
y
Adjust
culture medium to pH 6.0.
y
Dispense 15 mL
y
Transf er
in a 50
mL
Er lenmeyer flask and autoclave for 15 min at 121OC.
a loo pful of Lactobacillus culture f r o m agar slant into the first
medium
and incubate for 12-14 h at 36 °C in incubator shaker at 200 rpm. y
Prepare another f er mentation medium of volume 100 mL in 250
mL
and
O
autoclave for 15 min at 121 y
Transf er
C.
2 ml of the inoculum to the flask and incubate for 12-14 h to reach the
exponential gr owth at shak ing 200 rpm at 36 °C.
B) Fermentation:
y
Prepare 30 g/L of cor n steep liquor, 75 g/L of glucose, 1.5 g/L of yeast extract, 2g/L of (NH4)2HPO4, and 0.1 g/L of MnSO4 in 1L of distilled water.
y
Adjust
f er mentation medium to pH 6.0.
y
A
y
Transf er 1.35 L
2 L tank bioreactor is used for this f er mentation. of f er mentation medium into bioreactor and ready to autoclave O
for 15 min at 121 y
Transf er 150 ml
y
Dur ing
C.
of innoculum into bioreactor.
all f er mentation, agitation speed is fixed at 200 rpm and the tem perature
within the f er menter was contr olled at 36 °C and pH at 6.0. y
Calibrate
y
The
the pum p rate before starting any continuous f er mentation.
sam ples were removed aseptically at regular intervals every 4 hours until 24
hours for further analyses.
C) Analysis y
Lactic
acid was quantified by HPLC analysis cou pled with a UV var ia ble
wavelength detector set to 210 nm. y
An Aminex
HPX-87H ion-exclusion column was eluted with 5 mM sulfur ic acid
solution at 0.6 mL/min, and the column te m perature was maintained at 35 °C. y
Cell
gr owth was deter mined tur bidimetr ically by a spectr o photometer at 660 nm,
and the values thus obtained were then converted to dry cell mass via calculation with the appr o pr iate standard curve.
