Cholesterol Reducing Effects of Lactobacillus Spp CHOLESTEROL REDUCING EFFECTS OF Lactobacillus spp. ISOLATED FROM BREAST MILK OF LACTATION MOTHER. SUHANIS NADIA BINTI SALLEH CHAPTER 1 INTRODUCTION Background of the study Cholesterol is the precursor of primary bile salts formed in the liver and store as conjugated bile salts in gall bladder to be release in digestive tract. (Corzo & Gilliland, 1999). Lipid and cholesterol rich food intake act as the main factor in increasing of heart disease (Anandharaj & Sivasankari, 2014). Thus, it is important to reduce cholesterol as prevention to cardiovascular disease. (Yildiz et. al, 2011). Even though pharmaceutical agent or therapy exists for hypercholesterolemia treatments, they are expensive and may produce side effect. (Schuster, 2004). Due to the reason, non pharmaceutical approaches which yield cholesterol reduction were examined and probiotics are one of several approaches that have been used (Anandharaj & Sivasankari, 2014). Problem statement 1.3 Research Objective 1.3.1 General objective To investigate the cholesterol reducing property of Lactobacillus spp. isolated from breast milk of lactation mother . 1.3.2Specific objective 1.3.2.1 To isolate Lactobacillus spp. from breast milk of lactation mother. 1.3.2.2 To identify Lactobacillus spp. isolated from breast milk of lactation mother. 1.3.2.3 To determine cholesterol reducing property of Lactobacillus spp. isolated from breast milk of lactation mother. Research hypothesis 1.4.1 Study hypothesis There is significant difference between Lactobacillus spp. isolated from breast milk of different lactation mother on its cholesterol reducing property. 1.4.2 Null hypothesis There is no significant difference between Lactobacillus spp. isolated from breast milk of lactation mother on its cholesterol reducing property. 1.5 Scope and limitation of the study This study focusing on identification of bacteria and its properties and includes molecular technique. The scope of this study involves both phenotypic and genotypic characterization. Some limitations arise in this study. The cholesterol reduction assay which will be done in vitro to mimic the in vivo mechanism may not be totally similar with in vivo environment. 1.6 Significant of study Breast milk is a possible source of Lactobacillus strains but there are only few studies done on isolation of probiotic from human’s milk. (Anandharaj & Sivasankari , 2014 ; Martin et al., 2004). The reliability of cholesterol reduction by using probiotics for hypercholesterolemia treatments have gain increase of interest. (Jones et al. 2004 ; Lim et al. 2004). Even so, the findings are more on lactic acid bacteria strains among Western origin subject (Yildiz et al. 2011). Different result may be obtained from other population subject and this study may enhance the finding of probiotic strains that capable in cholesterol assimilation. CHAPTER 2 LITERATURE REVIEW CHAPTER 3 METHODOLOGY Proposed methodology (Descriptive) Ethical issues Study area The study will be conducted in the final year research laboratory of microbiology section at UiTM Puncak Alam. Most of the experiments will be conducted at the laboratory except for sequencing which will be send away. Sample collection is done outside the study area and will be store in the laboratory storage section. Sample collection Breast milk sample will be collected from volunteers in sterile container. Prior to collection, the breast is clean with sterile water and apply with chlorexidine to remove other normal flora. The sample will be store on ice until delivery to the laboratory. The sample will then stored in -80oC if not directly use or for further use. For storage, the sample will previously transfer into several small vials to avoid multiple freeze and thaw. Isolation of Lactobacillus spp. 1ml of breast milk sample is transfer into 9ml of sterile saline (0.85% sodium chloride). The dilute samples will be plate on Man Ragosa Sharpe, MRS medium. The plate is incubate at 37oC for 24 to 48 hour in anaerobic condition. Identification of Lactobacillus spp. Isolated Lactobacillus spp. will be confirm based on growth on MRS medium, colony morphology, Gram staining, and catalase reaction. The isolated colony will be proceed with subculture to obtain pure culture. Further species identification will be performed by carbohydrate fermentation pattern using API 50 CHL test strip. The result is analyze using API LABTM PLUS software. MRS broth medium containing 20% glycerol is use to preserve the pure cultures and store at -80oC. PCR amplification of 16S rDNA and sequencing Modified method of Smoker and Barnum (1988) will be conducted for DNA isolation. The 16S rDNA will then amplify in thermocycler by 30 cycles which include denaturation at 940C for 30s, annealing at 56oC for 30s and elongation at 720C. The PCR result will be separated on gel electrophoresis to check for the purity and of the amplicon. The amplified rDNA will be purified with PCR purification kit and send for sequencing. Phylogenetic analysis Cholesterol reducing assay Statistical analysis The data will be collected in triplicate and will be analysed by SPSS software. Data will be expressed as mean and standard deviation. One way ANOVA test with significance level p < 0.05 will be used to determine the significant difference between means. Proposed methodology (Flow chart) 5.0 Expected outcomes For isolation and identification of Lactobacillus spp., various species may be identified. Generally, they are expected to be catalase negative, gram positive, rods or cocci. Results on API 50 CHL will confirm the specific species. In PCR amplification, there will be presence of bands of specific base pair for Lactobacillus spp. after the amplicons separated on the agarose gel. As for cholesterol reducing assay, there will be species which show cholesterol reducing property and the species with the most significant reduction of cholesterol will be identified. 6.0 Financial implications 7.0 Ganntt chart Work plan 2014 (September – December) Months Work plan September October November December Weeks 1 2 3 4 5 6 7 8 9 10 11 12 13 14 Briefing about final year project Meeting and discussion with supervisor Preparation for research proposal Submission of research proposal Research proposal assesment Identified research material Collection of research material Learn laboratory technique on research proposal Work plan 2015 (March – July) Months Work plan March April May Jun Weeks 1 2 3 4 5 6 7 8 9 10 11 12 13 14 Laboratory works/ data analysis Preparation of thesis Submission complete draft thesis Preparation for poster presentation Final draft thesis / thesis final editing Submission of thesis Work plan 2015 (March – June) Months Work Plan March April May June Weeks 1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16 Laboratory works/ data analysis Preparation of thesis Submission complete draft thesis Preparation for poster presentation Final draft thesis / thesis final editing Submission of thesis

CHOLESTEROL REDUCING EFFECTS OF Lactobacillus spp. ISOLATED FROM BREAST MILK OF LACTATION MOTHER.

SUHANIS NADIA BINTI SALLEH

CHAPTER 1

INTRODUCTION

Background of the study

Cholesterol is the precursor of primary bile salts formed in the liver and store as conjugated bile salts in gall bladder to be release in digestive tract. (Corzo & Gilliland, 1999). Lipid and cholesterol rich food intake act as the main factor in increasing of heart disease (Anandharaj & Sivasankari, 2014). Thus, it is important to reduce cholesterol as prevention to cardiovascular disease. (Yildiz et. al, 2011). Even though pharmaceutical agent or therapy exists for hypercholesterolemia treatments, they are expensive and may produce side effect. (Schuster, 2004).

Due to the reason, non pharmaceutical approaches which yield cholesterol reduction were examined and probiotics are one of several approaches that have been used (Anandharaj & Sivasankari, 2014).

Problem statement

1.3 Research Objective

1.3.1 General objective

To investigate the cholesterol reducing property of Lactobacillus spp. isolated from breast milk of lactation mother .

1.3.2Specific objective

1.3.2.1 To isolate Lactobacillus spp. from breast milk of lactation mother.

1.3.2.2 To identify Lactobacillus spp. isolated from breast milk of lactation mother.

1.3.2.3 To determine cholesterol reducing property of Lactobacillus spp. isolated from breast milk of lactation mother.

Research hypothesis

1.4.1 Study hypothesis

There is significant difference between Lactobacillus spp. isolated from breast milk of different lactation mother on its cholesterol reducing property.

1.4.2 Null hypothesis

There is no significant difference between Lactobacillus spp. isolated from breast milk of lactation mother on its cholesterol reducing property.

1.5 Scope and limitation of the study

This study focusing on identification of bacteria and its properties and includes molecular technique. The scope of this study involves both phenotypic and genotypic characterization. Some limitations arise in this study. The cholesterol reduction assay which will be done in vitro to mimic the in vivo mechanism may not be totally similar with in vivo environment.

1.6 Significant of study

Breast milk is a possible source of Lactobacillus strains but there are only few studies done on isolation of probiotic from human’s milk. (Anandharaj & Sivasankari , 2014 ; Martin et al., 2004). The reliability of cholesterol reduction by using probiotics for hypercholesterolemia treatments have gain increase of interest. (Jones et al. 2004 ; Lim et al. 2004). Even so, the findings are more on lactic acid bacteria strains among Western origin subject (Yildiz et al. 2011). Different result may be obtained from other population subject and this study may enhance the finding of probiotic strains that capable in cholesterol assimilation.

CHAPTER 2

LITERATURE REVIEW

CHAPTER 3

METHODOLOGY

Proposed methodology (Descriptive)
1. Ethical issues
2. Study area

The study will be conducted in the final year research laboratory of microbiology section at UiTM Puncak Alam. Most of the experiments will be conducted at the laboratory except for sequencing which will be send away. Sample collection is done outside the study area and will be store in the laboratory storage section.

Sample collection

Breast milk sample will be collected from volunteers in sterile container. Prior to collection, the breast is clean with sterile water and apply with chlorexidine to remove other normal flora. The sample will be store on ice until delivery to the laboratory. The sample will then stored in -80^oC if not directly use or for further use. For storage, the sample will previously transfer into several small vials to avoid multiple freeze and thaw.

Isolation of Lactobacillus spp.

1ml of breast milk sample is transfer into 9ml of sterile saline (0.85% sodium chloride). The dilute samples will be plate on Man Ragosa Sharpe, MRS medium. The plate is incubate at 37^oC for 24 to 48 hour in anaerobic condition.

Identification of Lactobacillus spp.

Isolated Lactobacillus spp. will be confirm based on growth on MRS medium, colony morphology, Gram staining, and catalase reaction. The isolated colony will be proceed with subculture to obtain pure culture. Further species identification will be performed by carbohydrate fermentation pattern using API 50 CHL test strip. The result is analyze using API LAB^TM PLUS software. MRS broth medium containing 20% glycerol is use to preserve the pure cultures and store at -80^oC.

PCR amplification of 16S rDNA and sequencing

Modified method of Smoker and Barnum (1988) will be conducted for DNA isolation. The 16S rDNA will then amplify in thermocycler by 30 cycles which include denaturation at 94⁰C for 30s, annealing at 56^oC for 30s and elongation at 72⁰C. The PCR result will be separated on gel electrophoresis to check for the purity and of the amplicon. The amplified rDNA will be purified with PCR purification kit and send for sequencing.

Phylogenetic analysis
Cholesterol reducing assay

Statistical analysis

The data will be collected in triplicate and will be analysed by SPSS software. Data will be expressed as mean and standard deviation. One way ANOVA test with significance level p < 0.05 will be used to determine the significant difference between means.

Proposed methodology (Flow chart)

5.0 Expected outcomes

For isolation and identification of Lactobacillus spp., various species may be identified. Generally, they are expected to be catalase negative, gram positive, rods or cocci. Results on API 50 CHL will confirm the specific species. In PCR amplification, there will be presence of bands of specific base pair for Lactobacillus spp. after the amplicons separated on the agarose gel. As for cholesterol reducing assay, there will be species which show cholesterol reducing property and the species with the most significant reduction of cholesterol will be identified.

6.0 Financial implications

7.0 Ganntt chart

Work plan 2014 (September – December)

Months Work plan	September	October	November	December
Weeks
1	2	3	4	5	6	7	8	9	10	11	12	13	14
Briefing about final year project
Meeting and discussion with supervisor
Preparation for research proposal
Submission of research proposal
Research proposal assesment
Identified research material
Collection of research material
Learn laboratory technique on research proposal

Work plan 2015 (March – July)

Months Work plan	March	April	May	Jun
Weeks
1	2	3	4	5	6	7	8	9	10	11	12	13	14
Laboratory works/ data analysis
Preparation of thesis
Submission complete draft thesis
Preparation for poster presentation
Final draft thesis / thesis final editing
Submission of thesis

Work plan 2015 (March – June)

Months Work Plan	March	April	May	June
Weeks
1	2	3	4	5	6	7	8	9	10	11	12	13	14	15	16
Laboratory works/ data analysis
Preparation of thesis
Submission complete draft thesis
Preparation for poster presentation
Final draft thesis / thesis final editing
Submission of thesis

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