Assessment of Physico-Chemical and Microbial Quality of Sugarcane Juice Sold by Street Vendors in Three Regions of Bangladesh ()
1. Introduction
In City, there is high demand for fresh juices especially in summer during the months of March through August [1] . Most of the sugarcane juices were sold in road side shops, recreational areas (parks) and busy market places by street vendors. Sugar cane juices are nutritious drinks with great taste and health benefits [2] . Sugarcane juice is a common man’s refreshing beverage and it is sold at most of the public places at a reasonable prices. Drinking sugarcane juice instead of artificial and aerated drinks helps to improve the health of a person.
Unpasteurized juices are preferred by consumers because of the “fresh flavor” attributes and hence, in recent times, their demand has increased. It is nutritious and refreshing. It contains about 15% natural sugar and is rich in organic salts and vitamins. In most cases, sugarcane juice is not available in hygienic condition. At room temperature, sugarcane juice contains mainly mesophilic bacteria. At refrigerated condition, the growth is possible mainly due to psychrophilic bacteria [3] . Various pathogenic organisms like Escherichia coli, coliforms, enterococci, Salmonella spp., and Vibrio cholerae have been isolated from sugarcane juice by several workers [4] [5] . In our country, for fresh flavor, sugarcane juice was sold as unpasteurized condition. Especially unpasteurized juices have been shown to be a potential source of bacterial pathogens notably, Salmonella, E. coli O 157:H7 [6] [7] [8] .
Use of unhygienic water for dilution, prolonged preservation without refrigeration, unhygienic surroundings often have been shown to harbor bacterial pathogens notably Escherichia coli, Salmonella spp., Shigella spp., and Staphylococcus aureus of sugarcane juice [9] [10] . Changes in pH may also promote the growth of pathogens [11] . There is health risks associated with initial contamination of foods by pathogenic bacteria as well as subsequent contamination by vendors during preparation, handling and cross contamination [12] .
The major ingredients of the juice such as water, sugar, natural fruit pulp etc. may also carry some microbial contaminants. During the preparation, bare hands were used for handing the ice and sieving of juice. The utensils and glasses were washed just by dipping in the same water. Water used for juice preparation can be a major source of microbial contamination. Other factors can act as source of contamination such as use of improper handling, unhygienic water for dilution.
Considering the above requirements, this study was designed with the objectives of determining the microbial colony numbers and chemical parameters of sugarcane juices in Mymensing, Gazipur, Narayangonj and comparing the parameters among the juices of these 3 districts samples which influence the consumer to make decision whether the juice they drinking are safe or not and help them to make correct decision.
2. Materials and Methods
2.1. Study Design
An analytical study based on chemical and microbiological quality assessment with comparison between sugarcane juices of three areas. Sugarcane juices were collected from Gazipur, Mymensingh and Narayangonj areas. Samples were collected from 10 important places of Gazipur, Mymensingh and Narayangonj for each during October 2022 to September 2023. The samples analyses were conducted in the laboratory of Food Technology and Nutritional Science Department, Mawlana Bhashani Science and Technology University, Sanntosh, Tangail, Bangladesh (Table 1).
2.2. Physico-Chemical Analysis of Sugarcane Juice
2.2.1. Determination of Moisture Content
Moisture percentages of sugarcane juice were determined by oven drying method [13] . A crucible first washed and dried up. The weight of the crucible was taken. Then 9 ml of sample was taken in the crucible and weighted. Crucible plus sample is then placed in an oven heated at 105˚C for 4 hours. The sample plus crucible was placed in desiccators and weighted. Repeated this process until final weight reached to constant weight.
2.2.2. Determination of Ash Content
Ash percentages of sugarcane juice were determined by incineration of samples in a muffle furnace [14] . Nine ml of sample was taken in a crucible. The sample was heated at 105˚C for 3 to 4 hours. Sample was then heated in a muffle furnace at 600˚C for 3 to 4 hours. Sample was then cooled and ash content of the supplied sample was measured.
2.2.3. Determination of Total Soluble Solid (TSS)
Total solid contents of sugarcane juices were determined by oven drying method [13] . A previously weighed empty, dry and clean flat bottom aluminum cup was taken. Nine ml of sample was weighed out into the cup. The cup was then placed on a hot place at 180˚C, until the residue begins to turned light brown. For drying the cup was then placed into an oven operated at 100˚C for 10 - 15 minutes. After drying, sample was taken out from the oven and cooled in desiccators, for
5 minutes. Then the cup with the dried sample was weighed out carefully.
2.2.4. Determination of Total Sugar by Titration with Fehling’s Reagent
Total sugar estimation is the analyses of total sugar present in food item. 10 - 15 gm sample was taken in a volumetric flask then add 45% ethanol and boiled for 1 hour. Then cooled and make the volume 250 ml with 50% ethanol. Then evaporate the ethanol and transferred into a volumetric flash and then 5 ml clarifying solution 1 and 2 was added and filtered solution was used for free sugar analysis. 5 ml of 6.35N HCL was added in the 20 ml supernatant solution and hydrolyzed on a boiling water bath for 30 minutes. Cooled and added few drops of phenolphthalein and then neutralized with 40% and 0.1N NaOH. Filtered and make the volume 100 ml with distilled water and the solution was taken into a burette. Then titrate with 5 + 5 ml Fehling’s solution A and B with methyl blue indicator in a boiling temperature [15] .
Here X = result of first step, Y = result of second step and Z = result of third step.
2.2.5. Determination of Reducing Sugar by Titration with Fehling’s Reagent
Determination of reducing sugar is the analyses of free reducing sugar present in food item. 10 - 15 gm sample was taken in a volumetric flask then add 45% ethanol and boiled for 1 hour. Then cooled and make the volume 250 ml with 50% ethanol. Then evaporated the ethanol and transferred into a volumetric flash and finally add 5 ml clarifying solution 1 and 2 and filtered solution was used for free sugar analysis. 5 ml of Fehling’s solution 2 was taken in a conical flask and added same volume of Fehling’s solution 1. Just before use 50 ml of distilled water was added and heat on a hot plate. At the start of boiling point 2 - 3 drops of methyl blue was added and titrated with stock sugar solution [15] .
2.2.6. Estimation of Titrable Acidity
At first 10 ml sugarcane juice was taken in conical flask. If juice dark adds some distilled water but not more than 5 times. Then 3 - 5 drops phenolphthalein is added in the juice. Ensure the tap on the burette is shut and using a funnel pour the 0.1 M solution of NaOH into the burette until it reaches the zero mark. Slowly titrate the NaOH into the juice/water solution (with a 25 ml burette or an automatic burette). Using phenolphthalein as an indicator, the point of neutrality is reached when the indicator changes from colorless to pink. The indicator color must remain stable (persisting for 30 seconds) and be light pink when viewed over a white background [16] .
2.2.7. Determination of PH
Sension TM+ PH 31, PH meter were used for determination of PH. Checking the PH meter and make sure the PH meter has worked well. PH meter set in a dry place. Calibrate the meter containing a buffer solution of PH 4, PH 7 and PH 10. Whenever readings are taken correctly, ensure that the meter is worked correctly. After rinsing in distilled water, place the sample solution to be tested, then take the reading correctly [17] .
2.2.8. Microbial Analysis
Total Viable Count (TVC), Total Coliform Count (TCC) and Total Fungal Count (TFC) were for fruit juice, sherbet, ingredient water and waste water samples were done according to the method of The International Commission on Microbiological Specifications for Foods [18] . In this study, Nutrient Agar from OXOID Ltd., Basingstoke, Hampshire, England was employed. Ingredients of recommended quantities were weighted by electric balance and were dissolved in prescribed amount of distilled water. Prepare 300 ml nutrient agar media in a conical flask then the mixture was boiled to mixture the ingredients thoroughly. Clean and fresh glass ware used in the experiment. All glass wares like plate, pipette were sterilized in a hot oven (Model No.980435, made in Germany) at 180˚C for 2 hours. All kinds of media, solutions and glass bottles were sterilized at 15 P.S.I (Pounds per square inch) for 20 minutes at 121˚C in an autoclave (Model No. JSAC-50). 1 ml of the sugarcane juice was diluted with 9 ml of sterile buffered peptone water and mixed well (10−1 dilution). Serial dilutions were prepared and spread plate technique was used on solid media. Serial dilutions of samples were made up to 105 with sterile buffered peptone water. 0.1 ml of each dilution was evenly spread on the nutrient agar medium and incubated. Plates were screened for the presence of discrete colonies after incubation period and the actual numbers of bacteria were estimated as colony forming unit per ml (cfu/ml).
2.3. Statistical Analysis
All the experiments were done with replication and analyzed with mean through Microsoft Excel 2007.
3. Results
The study was conducted to compare the physicochemical and microbiological quality of sugarcane juice, 30 samples were collected from different areas of Mymensingh, Gazipur and Narayangonj. The objective of the study was to determine the chemical and microbiological quality of sugarcane juice which influence the consumer to make decision rather the juice they drinking are safe or not and help them to make correct decision.
3.1. The Physico-Chemical Analysis of Sugarcane Juice Collected from Different Areas of Mymensingh
Sugarcane juices collected from different vendors of Mymensingh areas and estimated the chemical parameters in the laboratory and plotted in the following Table 2 indicate that the highest value of moisture, PH, ash, total soluble solid and titrable acidity were found about 82.88%, 5.35, 0.57%, 17.48% and 0.465% respectively, where the lowest value were about 79.26%, 5.0, 0.16%, 9.48% and 0.205% respectively in Mymensing areas.
3.2. Physico-Chemical Analysis of Sugarcane Juice Collected from Different Areas of Gazipur
Following table represents the chemical analysis of sugarcane juice where, moisture content, PH measurement, ash content, total soluble solid, and acidity of Gazipur samples were determined.
Table 3 shows that the highest value of moisture, PH, ash, total soluble solid and titrable acidity were found about 84.33%, 5.90, 0.27%, 11.98% and 0.396% respectively, where the lowest value were about 81.22%, 4.92, 0.04%, 5.98% and 0.077% respectively in Gazipur areas.
3.3. Physico-Chemical Analysis of Sugarcane Juice Collected from Different Areas of Narayangonj
Following table represents the chemical analysis of sugarcane juice where, moisture
Table 2. Physico-chemical parameters of samples collected from Mymensingh.
content, PH measurement, ash content, total soluble solid, and acidity of Narayangonj samples were determined.
Table 4 indicate that the highest value of moisture, PH, ash, total soluble solid and titrable acidity were found about 83.45%, 5.9, 0.23%, 10.48% and 0.523% respectively, where the lowest value were about 80.48%, 4.29, 0.08%, 4.98% and 0.220% respectively in Narayangonj areas.
From Table 5 highest average value of ash and TSS found in Mymensingh region but it was lowest in moisture content with 81.17%. Highest moisture (82.69%) and pH (5.35) found in Gazipur region with a lowest average value of ash (0.15%) and tritable acidity (0.220%). The samples of Narayanganj contained highest acid value (0.371%) with lowest pH (4.97%) value. The reasons might be
Table 3. Physico-chemical parameters of samples collected from Gazipur.
Table 4. Physico-chemical parameters of samples collected from Narayangonj.
the: Sugarcane production system, land preparation, planting seasons, planting methods, types of soil and its composition, farming and manure system, irrigation and harvesting system. The delay in extraction of harvested sugarcanes is reported to cause some changes in the juice quality.
3.4. Microbial Analysis of Selected Sugarcane Juice at Different Areas
30 samples were collected from different areas of Mymensingh, Gazipur and Narayangonj and were examined for the microbial analysis.
Highest TFC (57.1 × 105 cfu/ml) and TCC (5.06 × 105 cfu/ml) value were found in Narayanganj samples and highest TVC (14.9 × 105 cfu/ml) found in Mymensingh region. All the values indicate that they all highly exceeded the maximum permitted value according to Gulf standard (2000). The reasons behind this huge amount of contamination were unhygienic water for dilution, high temperature, unhygienic surroundings, use of unhygienic utensils etc. In most cases, running water is not available at vending sites; hands and utensils washing are usually done in one or more buckets, and sometimes without soap (Table 6).
4. Discussions
In the 20th century, sugarcane has been successfully established as an important agriculture crop in Bangladesh. Fresh sugarcane juice is very popular as refreshing delicious drink all parts of our country and it is rarely available commercially in packaged form. Processing and marketing of sugarcane juice is limited by its
Table 5. Average comparison of physico-chemical properties among Mymensingh, Gazipur and Narayanganj samples.
Table 6. Average comparison of microbial analysis of selected sample for all areas.
rapid deterioration [19] .
Bacterial contamination of sugarcane juice may occur at different stages such as by roller drum crushers, collecting vessels, ice added to the juice, hands of the personnel and the filter. The delay in extraction of harvested sugarcanes is reported to cause some changes in the juice quality [20] . Use of unhygienic water for dilution, without cooling, unhygienic surroundings often have been shown to harbor bacterial pathogens notably Escherichia coli, Salmonella spp., Shigella spp., and Staphylococcus aureus of sugarcane juice [21] . Serious health hazards due to the presence of pathogenic microbes in food can lead to food poisoning outbreaks. Many outbreaks of food borne diseases have been reported due to consumption of unpasteurized and contaminated juices [22] . Urging from this point present study carried out to determine the microbial load of sugarcane juice used by street vendors in Mymensingh, Gazipur and Narayangonj city and results were discussed below. From Table 2, we can see that the highest and lowest values of moisture, pH, ash, total soluble solid, reducing sugar, total sugar, titratable acidity for Mymensingh samples were 82.88% - 79.26%, 5.35% - 5.0%, 0.57% - 0.16%, 17.48% - 9.48%, 3.7% - 2.56%, 21.9% - 7.9% and 0.465% - 0.205% respectively. From Table 3 for the chemical properties of Gazipur, the highest and lowest value of moisture, ph, ash, total soluble solid, reducing sugar, total sugar, titratable acidity for Gazipur samples were 84.33% - 81.22%, 5.9% - 4.92%, 0.270.04%, 11.98% - 5.98%, 3.06% - 2.1%, 12.2% - 6.56% and 0.396% - 0.077% respectively. From Table 4 for the chemical properties of Narayangonj, the highest and lowest value of moisture, pH, ash, total soluble solid, reducing sugar, total sugar, titratable acidity for Narayangonj samples were 83.45% - 80.48%, 5.23% - 4.29%, 0.22% - 0.08%, 8.98% - 4.98%, 3.10% - 2.4%, 13.12% - 7.06% and 0.523% - 0.231% respectively. Krishnakumar & Devadas (2013) found total soluble solid, total sugar, pH, titrable acidity ranged from 15% - 22%, 10% - 18%, 5.00% - 5.50% and 0.178% - 0.29% respectively which slightly mach with our present study [23] . According to Swaminathan (2001), moisture and reducing sugar ranged from 75% - 85% and 0.3% - 3.0% respectively that also has similarity with our present study [24] . In the present study, values found from Mymensing, Gazipur, and Narayangonj samples were different from each other. The reasons might be the: Sugarcane production system, land preparation, planting seasons, planting methods, types of soil and its composition, farming and manure system, irrigation and harvesting system & etc. It has been argued that there are various problems in estimating input output relationship using survey data, because of the variables are not controlled as they are in an experiment [25] . The recommended microbiological standards for any fruit juice; all numbers are as per ml of juice consumed [26] .
From the present study we found that the minimum and maximum range of Total viable count, total coli form count and total fungal count of sugarcane juice for Mymensing areas was ranged from 0.6 × 105 - 43.6 × 105 cfu/ml, 0.4 × 105 - 6.4 × 105 cfu/ml and 5.5 × 105 - 56.5 × 105 cfu/ml. For the Gazipur samples minimum and maximum range of Total viable count, total coli form count and total fungal count were 4.6 × 105 - 21.6 × 105 cfu/ml, 0.6 × 105 - 8.4 × 105 cfu/ml and 21.5 × 105 - 54.5 × 105 cfu/ml. For the Narayangonj samples minimum and maximum range of Total viable count, total coli form count and total fungal count were 3.6 × 105 - 36.6 × 105 cfu/ml, 0.00 × 105 - 8.4 × 105 cfu/ml and 32.5 × 105 - 68.5 × 105 cfu/ml. Table 7 indicates that, the highest and lowest average value of TVC, TFC and TCC was found 14.83 × 105 - 13.51 × 105 cfu/ml (Mymensingh-Gazipur), 57.00 × 105 - 41.95 × 105 cfu/ml (Narayangonj-Gazipur) and 4.98 × 105 - 3.8 × 105 cfu/ml (Narayangonj-Gazipur) respectively. According to Javed ali, Mohammad Siddique (2015), minimum and maximum range of Total viable count, total coliform and total fungal count were 2 × 102 - 2 × 104 cfu/ml, 2.3 - 1100 cfu/ml and 4 × 102 - 3 × 107 cfu/ml respectively, which is slightly similar with our present study. It is fact that all the samples analyzed were found to be contaminated with different bacteria is matter of concern. These juices are contaminated by various processes. Water used for juice preparation can be a major source of microbial contaminants [27] . If ice and source water used is of poor quality, harmful microorganisms may persist in cane juice. In most cases, running water is not available at vending sites; hands and utensils washing are usually done in one or more buckets, and sometimes without soap. Some of the juices are not efficiently protected against flies, which may carry food borne pathogens. There is health risks associated with initial contamination of foods by pathogenic bacteria as well as subsequent contamination by vendors during preparation, handling and cross contamination. Street vendors are mostly ignorant of good hygienic practices (GHP) and cause diarrheal diseases, which can increase the risk of street food contamination. Serious health hazards due to the presence of pathogenic microbes in food can lead to food poisoning outbreaks [28] . All of sugarcane juices in our present study were found to be unfavorable for consumption because about all of them showed exceeded acceptable range of microbial load. Negligence in city areas may result in serious contamination that ultimately represents a low quality product sold by vendors to the consumers. This not only suggests that these juices are not very hygienic, but it also puts customers at risk of food-borne illnesses. Thus, it can be shown that every sugarcane juice sample from vendors in Mymensingh, Gazipur, and Narayangonj that was analyzed included more bacteria than was considered safe for human consumption.
5. Conclusion
The present study was undertaken to evaluate the safety parameters of street
Table 7. Gulf Standard for Microbial Count.
vended sugarcane juices sold in different location of Mymensingh, Gazipur and Narayangonj city. In the study, 30 samples from these 3 areas were collected to estimate the physoco-chemical property and microbial analysis. Physico-chemical values found from Mymensing, Gazipur, and Narayangonj samples were different from each other. The reasons might be the: Sugarcane production system, land preparation, planting seasons, planting methods, types of soil and its composition, farming and manure system, irrigation and harvesting system & etc. All sugar cane juices collected from the areas of Mymensingh, Gazipur and Narayangonj were highly contaminated with harmful microbes. Total bacterial count in the most of the juice sample was higher than the standard permitted value. Highest viable count was found in Gazipur. Lowest viable count was found in Narayangonj. Most of the samples showed equal or higher count than the permitted value. Water used for juice preparation can be a major source of microbial contaminants. If ice and source water used is of poor quality, harmful microorganisms may persist in cane juice. In most cases, running water is not available at vending sites; hands and utensils washing are usually done in one or more buckets, and sometimes without soap.
6. Limitations of the Study
At the time of conducting the study, several minor problems were experienced. The limitations of the study are given below:
· The effective time allowed to complete this study was not enough due to some uncontrollable variables which have squeezed our total effective time period.
· Sophisticated laboratory equipment and proper packaging materials is mandatory for any secure output of study.
· There were lacking in the laboratory supports and it was one of the limitations that handicappsd us to carry out extensive experiments.
· Costs with this type of work are significant. So without any financial assistance, it would be very difficult to carry forward these types of empirical project in practice.
Acknowledgements
We are thankful to the technical members of the Department of Food Technology and Nutritional Science, MBSTU for supportive assistance and gratitude to the Ministry of Science and Technology (MOST), Bangladesh for financial support to complete this project work.
NOTES
*These authors contributed equally to the present work and shared first authorship.
#Corresponding author.