The assessment of microencapsulated Lactobacillus plantarum survivability in rose petal jam and the changes in physicochemical, textural and sensorial characteristics of the product during storage

Fateme Shoaei; Ali Heshmati; Reza Mahjub; Amir Daraei Garmakhany; Mehdi Taheri

doi:10.1038/s41598-022-10224-w

. 2022 Apr 13;12:6200. doi: 10.1038/s41598-022-10224-w

The assessment of microencapsulated Lactobacillus plantarum survivability in rose petal jam and the changes in physicochemical, textural and sensorial characteristics of the product during storage

Fateme Shoaei ¹, Ali Heshmati ^1,^✉, Reza Mahjub ², Amir Daraei Garmakhany ³, Mehdi Taheri ¹

PMCID: PMC9007973 PMID: 35418196

Abstract

The present study aimed to develop a probiotic rose petal jam containing microencapsulated L. plantarum. The attributes of L. plantarum microcapsules and bacteria viability in simulated gastrointestinal conditions and jam were assessed. In addition, L. plantarum effects on physicochemical, textural and sensorial properties of jam were studied. The microencapsulation yield, diameter, and zeta potential value of the microcapsules ranged from 90.23 to 92.75%, 14.80–35.02 µm, and − 16.83 to − 14.71 mV, respectively. The microencapsulation process significantly increases the survival of L. plantarum in simulated gastrointestinal tract and jam. In jam samples containing L. plantarum microencapsulated with 2% sodium alginate and 3.5% or 5% Arabic gum and stored for 90 days, the bacterial count was higher than the acceptable level (10⁶ CFU/g). While there was no significant difference (P > 0.05) between physicochemical characteristics of non-probiotic and probiotic jams, taste and overall acceptance scores of microencapsulated probiotic jams were higher. The microencapsulation of L. plantarum in sodium alginate (2%) and Arabic gum (5%) and its inoculation into rose petal jam could yield a new probiotic product with increased health benefits.

Subject terms: Biological techniques, Microbiology

Introduction

Jam preparation has been one of the most common and low-cost methods for preserving fruits and supplying them in the off season¹. According to Iranian standards, jam is defined as an intermediate-moisture product with a total soluble solids (TSS) content of 65°Brix (depending on the type of fruit used) of at least 20–35%^1,2. Jams are a good source of energy, carbohydrates, and fiber and contain low levels of fat. They can be produced from various types of fruits. Rose petal jam is one of the highest consumed jams in Iran and in some other countries, including India³.

Rosa damascena Mill., known as Damask rose, belongs to the Rosaceae family⁴. In Iran, Damask rose is known as Gole Mohammadi⁵. It is utilized in the perfume, medicine, and food industries. Jam is the most important products prepared using Damask rose^3,5. Rose petal jam is used as a tonic and laxative. It is a good source of powerful antioxidants and has various health benefits, e.g., it helps alleviate dysmenorrhea and fluid retention⁶.

At present, due to consumer awareness regarding the benefits of functional foods, the demand for the production and supply of these products is increasing⁷. Probiotics are one of the most important functional foods; they are live microorganisms that have beneficial effects on host health when consumed in sufficient amounts^8,9. The number of viable probiotic cells at the time of consumption should be more than 10⁶ colony-forming unit (CFU)/g to exert a health benefit to humans¹⁰. Probiotics reduce the risks conferred by mutagens and carcinogens, improve lactose tolerance and the intestinal flora, and strengthen the immune system^11,12. Most probiotics used in foods belong to the genera Lactobacillus and Bifidobacterium¹³.

Probiotics are mainly added to dairy products. However, given the presence of cholesterol in milk and the lactose intolerance and sensitivity of some people to dairy products, non-dairy probiotic products, such as cereal, legume, fruit, and vegetable based foods and drinks, have been developed^14,15. Therefore, the addition of probiotics to plant foods can be a suitable alternative for the consumption of these bacteria in vegan diet and people who cannot consume dairy products^14,16. Plant-based probiotics are cheaper sources and contain various phytochemicals¹⁶.

When probiotics are inoculated into a new foodstuff or drink, it is important to ensure that they preserve their viability during storage. The viability of probiotics depends on the oxygen level, final acidity of the product, water activity (AW), storage temperature, and presence of antimicrobial compounds^13,17. Therefore, microencapsulation is an important method for increasing the survival of probiotics in foods during storage and transfer through the gastrointestinal tract¹⁸ From a microbiological point of view, microencapsulation is the coating of probiotics with various substances, including gums, maltodextrin, starch, chitosan, and gelatin, etc. to protect them from the external environment¹⁹.

There are few studies about probiotic jam production. Only one study investigated the viability of probiotic bacteria inoculated into peach jam¹⁰ and there is no published information about the production of probiotic rose petal jam. The viability of probiotics in jam could be reduced during storage because the low AW of the product and storage conditions (mostly at room temperature) could result in the death of probiotic bacteria. The aim of the present study was to assess the survival of free/microencapsulated L. plantarum in simulated gastrointestinal conditions and jam. In addition, probiotic effects on the physicochemical, textural, and sensorial characteristics of jam during storage at different temperatures were investigated.

Materials and methods

Materials

Sodium alginate and Arabic gum were obtained from Sigma Aldrich (St-Louis, USA). MRS agar and MRS broth were produced by Liofilchem (Roseto degli Abruzzi, Italy). Sodium hydroxide (NaOH), calcium chloride (CaCl₂), potassium monophosphate (H₂PO₄), hydrochloric acid (HCl) and sodium citrate, pepsin and pancreatin and other chemicals were also purchased from Merck (Darmstadt, Germany). Lyophilized L. plantarum (ATCC 8014, PTCC: 1058), was bought from the Persian Type culture collection (Tehran, Iran).

Preparation of viable cells and suspension of L. plantarum

Lyophilized L. plantarum was reactivated twice in MRS broth at 37 °C for 24 h. The cell suspension was centrifuged (ROTOFIX 32A, Hettich, Germany) at 4000 × g for 6 min at 4 °C. After the removal of the supernatant, 0.85% sterile normal saline solution was added and mixed to obtain free L. plantarum suspension^18,20. The bacterial number in this solution that was counted according to the previous study¹³ was equal to 6 × 10¹⁰ CFU/mL.

Microencapsulation of L. plantarum

The microencapsulation of L. plantarum by sodium alginate and Arabic gum was performed according to previous studies with some modifications^21,22. First, a sodium alginate solution (1, 1.5 and 2% w/v) was prepared and sterilized (121 °C for 15 min). Two mL of L. plantarum suspension (6 × 10¹⁰ CFU/mL) was inoculated into 98 mL of sodium alginate solution and blended gently using a magnetic stirrer²¹. The obtained suspension was then dropped into sterile calcium chloride (1 L, 2% w/v) from a height of 20 cm through a sterile disposable needle with a diameter of 0.4 mm. After 20 min, beads were acquired by filtration through Whatman filter paper (No. 4) and washed with sterile deionized water²¹.

For second-layer formation on beads, Arabic gum was utilized. Arabic gum (2, 3.5 and 5% w/v) was dispersed in hot distilled water (75 °C) and stirred (600 RPM, 30 min) until complete dissolution. Afterwards, the beads were immersed into the sterilized Arabic gum (100 mL) and stirred for 30 min at 600 RPM¹⁸. Then they were transferred into the sterile glass, pre-frozen (− 20 °C, 2.5 h), placed in the freezer (− 70 °C, 12 h) for complete freezing, and dried in vacuum-freeze dryer equipment (operon, Hwanggeum, Korea) at − 55 °C for 24 h²⁰. The obtained beads or microcapsules were collected in polyethylene bags and stored at 4°C²⁰.

Microencapsulation efficiency

The efficiency of microencapsulation was determined according to the method suggested by Arepally and Goswami, 2019 and Chen et al. 2017.

Microencapsulation efficiency = \frac{(N \times M)}{(N 0 \times V)} \times 100

where N is L. plantarum count (log CFU/g) in microcapsules, M is the mass of the obtained microcapsule, N₀ is L. plantarum count (log CFU/g) in cell suspension, V is the volume of L. plantarum suspension used for microencapsulation preparation^18,23.

For L. plantarum count (log CFU/g) in microcapsules, 1 g of dried powder of the microencapsulated L. plantarum was suspended in 99 mL of sodium citrate (2%) solution²¹. The suspension was homogenized (100 RPM, 20 min, 37 ^○C) by a shaker (Teifazma, Tehran, Iran). After the preparation of appropriate dilutions (tenfold serial dilutions in 0.85% saline solutions), one mL of each dilution was plated on MRS agar. L. planetarium was counted after incubation in anaerobic jar (Gas Pack, Anaerogen TM, Oxoid) at 37 °C for 24 h. Plates containing 30–300 colonies were counted, and L. plantarum number for each was recorded and reported as log CFU/g of dried powder²⁰.

The measurement of microcapsules size

The average size of the microcapsules was determined by a laser light diffraction Malvern (Malvern Instruments, Malvern, Worcestershire, UK) instruments²⁴.

The measurement of zeta potential

The zeta potential of microcapsules diluted to 0.001% with deionized water was measured²⁵ with zetasizer particle size analyzer (Malvern Instruments Ltd. Malvern, Worcestershire, UK).

Morphology of microcapsules

The morphology of microcapsule was measured with a scanning electron microscopy (SEM) (JEOL Co., Akishima, Japan) according to procedure suggested by previous study²⁵.

Measurement of moisture and AW of microcapsules

The moisture content of microcapsules was determined gravimetrically in oven (Shimaz Inc., Tehran, Iran) at 105 °C for 24 h. AW was measured at 25 ± 1 °C using a water activity meter (LabMaster. aw, Novasina, Switzerland). Before AW measurement of microcapsules, the equipment was calibrated with distillate water for result accuracy¹⁸.

The preparation of simulated gastric and intestinal juice

The simulated gastric juice (SGJ) was prepared according to the method suggested by Annan et al.²⁶ Therefore, pepsin (0.3% w/v) was added into sterile sodium chloride solution (0.2% w/v), and its pH was adjusted to approximately 2 with HCl (0.1 N) and filtrated through a membrane (0.45 µm, Millipore, Spain) for sterilizing.

For simulated intestinal juice (SIJ) preparation, pancreatic (0.1% w/v) and bile salts (0.45% w/v) were added into citrate sodium (2%). The mixture’s pH was adjusted to 7.4 with NaOH (0.1 N) and sterilized by filtration through a membrane (0.45 µm Millipore, Spain). Both gastric and intestinal juices were prepared and used daily²⁶.

Survival assay of free and microencapsulated L. Plantarum after sequential incubation in simulated gastrointestinal conditions

To assess the viability of L. plantarum under a simulated gastrointestinal condition (SGC), the applied method was similar to that used by Fareez et al.²⁸ and Krasaekoopt and Watcharapoka²⁷, with some modifications. Free L. plantarum suspension (1 mL) or microencapsulated L. plantarum (1 g) was added into falcon tubes containing SGJ (9 mL) and placed into a shaker incubator (100 RPM, 37 °C) for different times (0, 30, 60, 90, 120 and 180 min)²⁸. After neutralizing with NaOH solution (0.1 N), the treated L. plantarum was removed from the SGJ by centrifugation (4,000 g, 10 min). The beads and cells were washed once with sterile distilled water and transferred into in a falcon tube containing SIJ (10 mL). The tubes were placed in a shaker-incubator at 37 °C for 180 min. Furthermore, beads and cells were removed by centrifugation (4000 g, 10 min), dissolved in sodium citrate (2%), and cultured as explained in the above Section²⁰.

The preparation of probiotic rose petal jam

A schematic diagram of the production stages of the rose petal jam is provided in Fig. 1. In summary, 50 g of dried rose petals were placed in boiling water for 3 min to remove the bitter taste. Then, the samples were placed in cold water for 5 min. In the final step, the samples were poured over a sieve to drain out the water. Debittered rose petal jam samples were placed in a stainless steel pot. Syrup (a 50% sugar solution) was added and heated for 30 min. Finally, 1 tablespoon of lemon juice was added. When the samples’ temperature reached 45 °C, they were poured into glass containers. One mL of free L. plantarum suspension (6 × 10¹⁰ CFU/mL) or one g of micencapsulated L. plantarum (approximately 1.2 × 10¹⁰ CFU/g) was added into 100 g of jam. The samples were kept at 2 temperature conditions (4 and 25 ^○C) for 90 days^10,29. Because L. plantarum microencapsulated in sodium alginate (1%) and Arabic gum (2, 3.5 and 5%) had low survival under a simulated gastrointestinal condition, they were not inoculated in the jam. The photos of probiotic and non-probiotic rose petal jam were shown in Supplementary Fig. S1.

The diagram of probiotic rose petal jam production.

Enumeration of L. Plantarum in jam

One g of jam samples stored for 1, 15, 30, 45, 75, and 90 days at room or refrigerator temperature was added into a falcon tube containing 9 mL peptone water and stirred. After preparing of serial (tenfold) dilutions, the number of bacteria was counted by a pour plate method using MRS agar. Plates were placed in an anaerobic jar and incubated at 37 °C for 24 h²⁹.

The assessment of physicochemical, textural and sensorial characteristics of probiotic rose petal jam

Determination of TSS

The TSS value of rose petal jam samples was measured by the digital refractometer (Krüss Optronic GmbH, Hamburg, Germany) at ambient temperature (20 °C) and expressed in °Brix².

The measurement of titratable acidity

The acidity of rose petal jam specimens was determined by titrating with sodium hydroxide solution (0.1 N) in the presence of phenolphthalein indicator and expressed as citric acid percentage².

The pH was directly determined by pH meter (Century, Model CP931, Bangalore, India).

The measurement of total non-reducing sugars

Total non-reducing sugar percentage of the rose petal jam was determined by the Lane and Eynon method³⁰.

The color evaluation

A color measurement was performed similar to that carried out in our previous study³¹. Rose jam samples were placed on the floor of an aluminum dark chamber with 30 × 40 × 40 cm dimensions. Four 60-W halogen lamps were in the corners of the chamber. Photos were taken with a camera (Canon, Kanagawa, Japan). The color parameters including L* (brightness), a* (red-green), b* (yellow-blue) of the jam were determined using Photoshop 7.0 software.

The evaluation of texture and viscosity

Viscosity and texture properties including firmness, cohesiveness and chewiness were measured using a texture analyzer (Zwick, Ulm, Germany). Texture analysis was carried out using a back extrusion test in 2 cycles. Jam samples were poured into plastic containers 50 mm in height. A cylindrical probe (20 mm in diameter) was applied to compress the sample to a 25 mm depth with a speed of 40 mm/min³².

The sensory evaluation

The sensory properties (taste, odor, appearance, and overall acceptability) of the rose petal jam were evaluated according to the hedonic scale of nine points (from 9 = like extremely to 1 = dislike extremely). Trained panelists (15 men and 15 women aged from 18 to 45 years old) were used for sensory testing. The samples were kept at 20 °C temperature for 3 h and then examined for sensory properties³³. A number code was considered for each sample. Then, the samples were poured into a sterile plastic spoon and given to panelist with their code randomized order. The panelists rinsed their mouths after testing each sample. The mean sensory scores were used in the analysis.

Ethical approval

The protocol of the sensory experiments was approved by the Ethics Committee of Hamadan University of Medical Sciences (ethics code: IR.UMSHA.REC.1397.1030). Informed consent was obtained from human panelists for sensory evaluation. All methods were performed in accordance with the relevant guidelines and regulations.

Statistical analysis

All the experiments were carried out in triplicate and their mean ± standard deviation were reported. The data were subjected to a one-way ANOVA and Duncan’s multiple range test to determine significant difference at the level of 95% using SPSS 22:0 Advanced Statistics (IBM; Armonk, NY, USA).

Results and discussion

Physicochemical properties of the microcapsules of L. plantarum

Microencapsulation efficiency

In this study, we used various levels of sodium alginate and Arabic gum for microencapsulation of L. plantarum. The statistical results showed the significant differences (P ≤ 0.05) in the efficiency of used various concentration levels (Table 1) so that the increased efficiency values was obtained at higher concentrations of sodium alginate (1.5 and 2%) and Arabic gum (2, 3.5 and 5%). Microencapsulation efficiency value ranged from 90.97 ± 4.68 to 98.86 ± 2.97%. In the previous study done by De Almeida Paula et al.²⁵ the microencapsulation efficiency of L. plantarum coated by Arabic gum and gelatin was reported as 97.8% that it was similar to our findings. The increment of sodium alginate and Arabic gum concentration lead to formation of microcapsules with the thicker layer and a higher probiotic count. On the other hand, a thicker coating could protect the probiotic viability during freeze-drying better than a thin coating³⁴. The high microencapsulation efficiency indicated that sodium alginate and Arabic gum were compatible matrices for microencapsulation of probiotics such as L. plantarum.

Table 1.

Physicochemical properties of the L. plantarum microcapsules.

Parameter	Al₁Ar₂	Al₁Ar_3.5	Al₁Ar₅	Al_1.5Ar₂	Al_1.5Ar_3.5	Al_1.5Ar₅	Al₂Ar₂	Al₂Ar_3.5	Al₂Ar₅
Encapsulation efficiency (%)	90.97 ± 4.68^c	91.75 ± 3.73^c	92.19 ± 5.6^c	92.3 ± 2.66^bc	93.42 ± 6.85^b	94.64 ± 4.97^b	95.23 ± 5.93^ab	97.97 ± 3.78^a	98.86 ± 2.97^a
Diameter (µm)	14.80 ± 1.23^c	19.30 ± 2.90^bc	21.71 ± 3.84^b	16.12 ± 1.42^c	21.26 ± 1.43^b	31.12 ± 3.56^a	16.92 ± 2.14^c	24.50 ± 3.21^b	35.02 ± 2.18^a
Zp (-mV)	15.81 ± 0.30^a	16.42 ± 0.36^a	16.30 ± 1.32^a	14.71 ± 0.76^a	16.83 ± 1.7^a	16.40 ± 0.95^a	15.82 ± 0.53^a	16.20 ± 2.27^a	15.77 ± 0.87^a
Moisture (%)	8.56 ± 2.22^a	7.70 ± 1.13^a	5.9 ± 2.06^b	7.8 ± 1.75^a	6.60 ± 1.18^ab	5.50 ± 3.08^b	7.87 ± 0.23^a	5.67 ± 1.53^b	4.38 ± 3.5^b
AW	0.18 ± 0.01^a	0.18 ± 0.01^a	0.16 ± 0.02^a	0.15 ± 0.00^ab	0.13 ± 0.02^b	0.12 ± 0.03^b	0.15 ± 0.04^ab	0.14 ± 0.39^ab	0.11 ± 0.05^b

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Values are expressed as mean ± standard deviation (n = 3). Means followed by different lowercase letters differ statistically in the same column (P ≤ 0.05). AlAr shows L. plantarum microencapsulated with levels of 1, 1.5 and 2% sodium alginate (Al) and 2, 3.5 and 5% Arabic gum (Ar).

Encapsulation efficiency impacts the final number of probiotics in food and their viability in the gastrointestinal tract^22,35. A previous study by Arepally and Goswami (2019) showed that the increasing Arabic gum concentration resulted in increased encapsulation efficiency, that it was similar to our results¹⁸.

Microcapsule size and morphology

The diameter of the prepared microcapsules in the current study ranged from 14.80 ± 1.23 to 35.02 ± 2.18 µm and depended on the sodium alginate and Arabic gum concentration (Table 1). Microcapsules more than 1000 µm in diameter had a negative impact on the sensory attributes of products. On the other hand, microcapsules with a size of less than 1 µm were unstable³⁶. Microcapsule size may affect different properties such as solubility, water activity, and the number of viable probiotic cells³⁷. The size of prepared L. plantarum microcapsules in the present study was small enough to avoid any negative effects on sensorial quality. According to the previous study, microcapsule size was directly proportional to hydrogel material viscosity: the higher viscosity lead to the larger particles size^38,39. Therefore, it seemed that increasing sodium alginate and Arabic gum concentrations resulted in enhanced viscosity of prepared solutions, which could cause an increase in microcapsule size.

Supplementary Figs. S2 and S3 depicts the morphology (at magnifications 50 × and 5000 ×) of L. plantarum microencapsulated with different levels of sodium alginate and Arabic gum. Due to the ionic bond between the carboxyl group of sodium alginate and calcium, the structure of the microcapsules became spherical. Sodium alginate was also placed as a first layer on a suitable substrate of the second layer. Increased concentrations of sodium alginate and Arabic gum led to a smoother microcapsule surface. Therefore, the microcapsules formed with 2% sodium alginate and 5% Arabic gum had the smoothest surface (Supplementary Fig. S2). A smooth surface increases the protective properties of microcapsules and increases probiotic cell survival (Kalita et al. 2018). Previous studies have found that the morphology of microcapsules depends on the type of coating and its concentration⁴⁰.

Zeta potential of microcapsules

As it can be seen in Table 1, the zeta potential value did not differ significantly (P > 0.05) among the different treatments. The zeta potential value ranged − 16.83 to − 14.71 mV. Sodium alginate and Arabic gum could be uniformly layered. The occurrence of carboxylic group of sodium alginate and Arabic gum created negative zeta potential³⁴ Lee and Chang (2020) found that high zeta potential values prevent aggregation of emulsion droplets⁴¹. In the present study, the amount of zeta potential was in the medium level, therefore it could lead to particle stability and preventing agglomeration.

Moisture content and AW of microcapsules

As shown in Table 1, the moisture content of prepared microcapsules ranged from 4.38 ± 3.50 to 8.56 ± 2.22%, indicating a favorable drying process. Moisture content affects the chemical and mechanical properties and storage stability (agglomeration) of microcapsules⁴². Our results showed that moisture content decreased with increasing Arabic gum and sodium alginate concentration. The high levels of Arabic gum and sodium alginate improved emulsion stability and surface tension and increased emulsion viscosity and caused moisture decrease. Arepally and Goswami (2019) showed the increasing of Arabic gum and maltodextrin concentration led to the moisture content reduction of capsules that these findings were similar to our results. The moisture content of the prepared probiotic microcapsules in various studies differed and was dependent on the type of coating materials and drying method⁴³. In all microcapsules, the amount of AW was less than 0.2. In general, microcapsules with AW < 0.1–0.2 are stable from microbiological and biochemical aspects⁴⁰. When AW is lower than 0.1, the probiotic death rate was increased due to oxidation of the membrane⁴⁴. In a study carried out by Fazilah et al.⁴⁵, AW level of microcapsules based on Arabic gum was lower than 0.3, which is approximately similar to our findings.

The survival of free and encapsulated L. plantarum during sequential incubation in simulated gastrointestinal conditions

The microencapsulation of L. plantarum within sodium alginate and Arabic gum had a significant effect (P ≤ 0.05) on its survivals increment during exposure to simulated gastrointestinal juice. By increasing incubation time of L. plantarum during exposure to simulated gastrointestinal juice, a continuous reduction in number of probiotic cells was observed (Fig. 2A). The highest (6.37 ± 0.10 log CFU/g) and lowest (1.46 ± 0.05 log CFU/g) of reduction were related to free L. plantarum and L. plantarum microencapsulated by 2% sodium alginate and 5% Arabic gum, respectively (Fig. 2B). The higher concentration of sodium alginate and Arabic gum resulted in thicker double-layer structure that could have greater protective impacts against the violent environmental factors such as simulated gastrointestinal conditions, therefore it could increase probiotic stability and viability⁴⁶.

(A) The survival (log CFU/g) of free and microencapsulated *L. plantarum* after incubation in simulated gastric juices for 0, 30, 60, 90, 120 and 180 min and sequentially in stimulated intestinal juice containing 0.6% bile salt solutions at 37 °C for 180 min. B: The total reduction value of the number of viable cells of *L. plantarum* after incubation in simulated gastric juices (180 min) and sequentially in stimulated intestinal juice (180 min) (B) Values are expressed as mean ± standard deviation (n = 3). In (A), Lowercase letters above columns indicate significant difference (P ≤ 0.05) among different treatments for the same storage period and uppercase letters above columns indicate significant difference (P ≤ 0.05) among different storage period for each treatment. In (B), lowercase letters above columns indicate significant difference (P ≤ 0.05) among different treatments. Free indicates free (non-microencapsulated) *L. plantarum*; and AlAr shows *L. plantarum* microencapsulated with levels of 1, 1.5 and 2% sodium alginate (Al) and 2, 3.5 and 5% Arabic gum (Ar).

The survival of L. plantarum during jam storage in different conditions

The results of L. plantarum survival during jam storage under different conditions are shown in Fig. 3. In all treatments, the count of L. plantarum decreased over time (Fig. 3A and B). The survival of free L. plantarum was much lower than the microencapsulated form. The low pH and AW of jam lead to probiotic death^17,47. However, microencapsulation protects probiotic against the mentioned conditions. The viability of L. plantarum in jam samples stored at room temperature was significantly (P ≤ 0.05) lower than those stored at refrigerator temperature. The high storage temperature causes the increment of cell metabolism and death of probiotic⁴⁸. The reduction level of free L. plantarum after 90 days of storage at refrigerator and room temperature was 4.63 ± 0.08 and 5.27 ± 0.35 log CFU/g, respectively (Fig. 3C and D). In jam samples containing L. plantarum microencapsulated with 2% sodium alginate and 3.5% or 5% Arabic gum, stored for 90 days at room or refrigerator temperature, the bacterial count was higher than the acceptable level (10⁶ CFU/g).

Changes in free and microencapsulated *L. plantarum* count (log CFU/g) during probiotic rose petal jam storage at 4 °C (A) and 25 °C (B). The total reduction value of the number of viable cells of *L. plantarum* after 90 days of storage at 4 °C (C) and 25 °C (D). Values are expressed as mean ± standard deviation (n = 3). In (A) and (B), lowercase letters above columns indicate significant difference (P ≤ 0.05) among different treatments for the same storage period and uppercase letters above columns indicate significant difference (P ≤ 0.05) among different storage period for each treatment. In (C) and (D), lowercase letters above columns indicate significant difference (P ≤ 0.05) among different treatments. Free indicates free (non-microencapsulated) *L. plantarum;* and AlAr shows *L. plantarum* microencapsulated with levels of 1.5 and 2% sodium alginate (Al) and 3.5 and 5% Arabic gum (Ar).

The count of free L. plantarum in jam stored for 30 days at refrigerator temperature was less than 10⁶ CFU/g. Our finding was similar to the study performed by Randazzo et al.¹⁰, where, the count of free L. ramensus in peach jam was less than 10⁶ CFU/g after 30 days of storage at refrigerator temperature.

As results show, the utilization of sodium alginate and Arabic gum for microencapsulation of L. plantarum could increase the viability of this bacteria in jam. Therefore, it is a suitable strategy for enhancing the viability of L. plantarum inoculated rose petal jam.

Effect of storage time and temperature on the physicochemical, textural and sensorial characteristics of probiotic and non-probiotic rose petal jam

pH and acidity

The acidity of the produced jams ranged from 0.44–0.65% (in citric acid) and the pH value ranged from 3.44 to 4.15 (Fig. 4A and B). In all the samples, pH significantly decreased during the storage period, while the acidity significantly increased (p ≤ 0.05). These findings were similar to the results reported in previous studies^49,50. There was no significant difference (P > 0.05) between the pH values and acidity percentages of the non-probiotic and probiotic jams stored for a given time. Therefore, the addition of free and encapsulated L. plantarum into rose petal jam has no effect on its pH and acidity. In contrast to our results, previous studies have reported that inoculation of probiotics into products, such as cake and juice, could change the pH and the acidity percentage during the storage period^51,52. The increment of acidity during probiotic jam storage was related to dissociation of organic acids over the time⁴⁹.

Changes in chemical properties of control (non-probiotic) and probiotic rose petal jams during storage in 4 °C and 25 °C. (A) Acidity; (B) pH; (C) Total soluble solids (TSS); (D) Total non-reducing sugar. C indicates control (non-probiotic) jam; Free indicates probiotic jam containing free (non-microencapsulated) *L. plantarum;* and AlAr shows probiotic jam containing *L. plantarum* microencapsulated with levels of 1.5 and 2% sodium alginate (Al) and 3.5 and 5% Arabic gum (Ar). T₄ and T₂₅ indicate storage time of 4 and 25 °C, respectively.

TSS

In all probiotic and non-probiotic jam samples, the amount of TSS increased during the storage period (Fig. 4C), although this increment was not significant (P > 0.05). There was no significant difference (P > 0.05) between TSS of the different treatments at a given temperature and time (Fig. 4C). During the storage period, due to conversion of insoluble constitutes to soluble substances, the amount of TSS increased⁵³.

Total non-reducing sugars

The amount of non-reducing sugar in the jam samples decreased during the storage period (Fig. 4D). There was no significant (P > 0.05) difference in the levels of non-reducing sugar of the probiotic and non-probiotic jam samples (P > 0.05). During the storage period, sucrose is hydrolyzed to glucose and fructose due to increased acidity¹⁰. The amount of non-reducing sugar that decreased during the storage period was also found in other jams, such as apricot jam and coconut jam^53,54, which is in agreement with the result of our study.

Color

The addition of the free and microencapsulated form of L. plantarum did not have a significant effect (P > 0.05) on the L^*, a^*, and b^* color parameters of the rose petal jam (Table 2). However, the brightness (L^* value) of the non-probiotic and probiotic rose petal jam samples decreased significantly during the storage period (P ≤ 0.05). There was no significant difference (P > 0.05) in the a^* and b^* color values of the samples stored at room temperature or those stored in the refrigerator, although their color values increased during the 90-day storage period. The reduction of the L^* value and the increment of the a^* and b^* color values during the storage period indicate that the sample darkened due to the formation of brown pigments as a result of the non-enzyme browning reaction⁵⁵. Previous studies have reported that probiotics did not change the color of the product⁵².

Table 2.

Changes in color (L^∗, a^∗, and b^∗) of plain and probiotic rose petal jams during storage in 4 °C and 25 °C.

Parameter	storage temperature (°C)	Storage time (day)	Treatment
Parameter	storage temperature (°C)	Storage time (day)	C	Free	Al_1.5Ar₂	Al_1.5Ar_3.5	Al_1.5Ar₅	Al₂Ar₂	Al₂Ar_3.5	Al₂Ar₅
L*	4	1	50.50 ± 1.73^Aa	49.75 ± 2.21^Aa	49.23 ± 0.89^Aa	51.33 ± 1.53^Aa	47.50 ± 10.47^Aa	45.25 ± 3.30^Aab	49.25 ± 0.96^Aa	52.25 ± 0.95^Aa
	25	1	49.50 ± 1.30^BAa	52.00 ± 4.76^Aa	52.36 ± 2.00^Aa	48.00 ± 7.74^Aa	49.50 ± 3.69^Aa	49.75 ± 1.70^Aa	47.75 ± 3.09^Aa	51.75 ± 0.96^Aa
	4	45	42.33 ± 9.61^Ab	43.33 ± 7.23^Ab	44.12 ± 0.98^Aab	44.67 ± 5.86^Aab	45.67 ± 0.58^Aab	42.33 ± 5.03^Aab	46.00 ± 3.47^Aa	45.00 ± 1.73^Aab
	25	45	45.00 ± 3.00^Aab	41.00 ± 4.35^Ab	45.78 ± 1.02^Aab	41.75 ± 13.22^Ab	46.00 ± 4.35^Aab	45.67 ± 1.71^Aab	43.33 ± 9.86^Aab	46.00 ± 2.00^Aab
	4	90	41.25 ± 2.87^Ab	38.50 ± 2.88^Aac	42.56 ± 3.45^Ab	41.00 ± 16.79^Ab	43.75 ± 5.25^Aab	40.75 ± 1.50^Ab	39.25 ± 1.50^Ab	42.25 ± 4.99^Ab
	25	90	40.25 ± 6.60^Ab	37.00 ± 1.82^Ac	40.87 ± 5.68^Ab	39.00 ± 1.82^Ab	42.25 ± 6.13^Ab	40.50 ± 5.00^Ab	35.25 ± 3.20^Ab	42.50 ± 7.76^Ab
a*	4	1	37.50 ± 4.12^Ac	42.00 ± 3.74^Aab	36.45 ± 1.25^Ac	37.00 ± 6.68^Ab	36.50 ± 5.25^Ab	37.75 ± 7.13^Ac	38.00 ± 1.15^b	38.33 ± 1.53^Ac
	25	1	39.50 ± 1.29^bAc	40.75 ± 0.96^Ab	37.05 ± 1.98^Ac	37.75 ± 6.13^Ab	42.25 ± 1.89^Aa	42.00 ± 2.16^Ab	37.50 ± 1.91^Ab	41.75 ± 2.98^Ab
	4	45	42.67 ± 7.57^Ab	41.67 ± 4.93^Aab	38.10 ± 2.06^Ac	42.25 ± 3.86^bA	43.75 ± 4.11^Aa	37.67 ± 1.15^Ac	42.67 ± 2.08^Aa	42.75 ± 3.77^Ab
	25	45	42.00 ± 2.94^Ab	39.67 ± 1.53^Ab	41.23 ± 3.61^b	49.67 ± 1.53^Aa	43.33 ± 5.13^a	45.33 ± 2.08^Aa	41.67 ± 5.78^Aa	43.33 ± 4.51^Ab
	4	90	44.50 ± 2.89^Ab	43.50 ± 2.64^Aa	46.25 ± 1.08^Aa	50.00 ± 2.65^Aa	44.33 ± 0.58^Aa	46.50 ± 1.29^Aa	43.75 ± 4.99^Aa	44.00 ± 0.00^Ab
	25	90	49.33 ± 3.06^Aa	46.00 ± 3.16^Aa	49.12 ± 2.35^Aa	48.75 ± 3.40^Aa	46.25 ± 2.50^Aa	47.75 ± 4.11^Aa	46.50 ± 1.73^Aa	49.25 ± 3.59^Aa
b*	4	1	42.00 ± 1.63^Aa	41.00 ± 4.04^Aa	38.02 ± 3.05^Ab	37.00 ± 7.35^Ab	36.25 ± 5.56^Ab	42.75 ± 3.50^Ab	38.25 ± 1.70^Ab	41.00 ± 1.41^Ab
	25	1	41.00 ± 0.81^Aa	44.00 ± 2.70^Aa	38.25 ± 4.15^ABb	38.75 ± 9.56^ABb	35.50 ± 4.51^Bb	45.00 ± 4.08^Aab	40.75 ± 3.40^Ab	44.50 ± 2.08^Ab
	4	45	44.00 ± 7.94^ba	43.67 ± 7.57^Aa	41.32 ± 2.56^Aa	41.00 ± 5.20^Ab	45.33 ± 0.58^Aa	45.67 ± 3.51^Aab	45.33 ± 3.79^Aa	44.67 ± 1.15^Ab
	25	45	43.00 ± 4.00^Aa	45.67 ± 3.21^Aa	42.65 ± 3.26^Aa	42.33 ± 2.08^Ab	45.67 ± 6.43^Aa	47.00 ± 3.00^Aa	42.00 ± 7.81^Aab	46.00 ± 3.60^Aab
	4	90	46.50 ± 6.19^Aa	45.75 ± 2.75^Aa	43.19 ± 5.86^Aa	48.00 ± 9.41^Aa	47.50 ± 6.65^Aa	50.50 ± 2.08^Aa	49.00 ± 5.09^Aa	49.50 ± 5.06^Aa
	25	90	45.50 ± 3.70^Aa	45.50 ± 1.29^Aa	42.78 ± 2.48^Aa	51.50 ± 3.10^Aa	47.25 ± 7.13^Aa	51.50 ± 5.19^Aa	47.50 ± 3.31^Aa	50.50 ± 8.50^Aa

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Values are expressed as mean ± standard deviation (n = 3). Means followed by different uppercase letters differ statistically within the same row (P ≤ 0.05). Means followed by different lowercase letters differ statistically within the same column (P ≤ 0.05). C indicates control (non-probiotic) jam; Free indicates probiotic jam containing free (non-microencapsulated) L. plantarum; and AlAr shows probiotic jam containing L. plantarum microencapsulated with levels of 1.5 and 2% sodium alginate (Al) and 3.5 and 5% Arabic gum (Ar).

Viscosity

The results indicated that the viscosity of all the samples was significantly increased during the storage period (P ≤ 0.05). The samples containing microencapsulated L. plantarum had a higher viscosity than the samples containing the free L. plantarum or those containing non-probiotics (Table 3). The viscosity was impacted by the storage conditions. The samples stored in the refrigerator had greater viscosity than those stored at room temperature. The increased pectin depolymerisation in high temperature results in viscosity reduction⁵⁶. The viscosity of jam depends on various factors, such as pH, TSS and the concentration of sugar, and pectin⁵⁷. In this study, samples containing greater concentration of sodium alginate and Arabic gum had higher viscosity. It seemed that the absorption of water by sodium alginate and Arabic gum during the storage period increases jam samples viscosity.

Table 3.

Changes in viscosity and texture properties of plain and probiotic rose petal jams during storage in 4 °C and 25 °C.

Parameter	Storage temperature (°C)	Storage time (day)	Treatment
Parameter	Storage temperature (°C)	Storage time (day)	C	Free	Al_1.5Ar₂	Al_1.5Ar_3.5	Al_1.5Ar₅	Al₂Ar₂	Al₂Ar_3.5	Al₂Ar₅
Viscosity (centipoise)	4	1	507.81 ± 45.23^Bd	512.45 ± 71.23^Bd	617.9 ± 50.18^Ad	623.93 ± 63.5^Ad	638.76 ± 65.15^Ad	655.87 ± 72.72^Ad	663.84 ± 96.26^Ad	670.83 ± 87.63^Ad
	25	1	437.5 ± 23.23^Be	445.23 ± 58.4^Be	553.88 ± 47.93^Ae	552.95 ± 60.98^Ae	566.25 ± 61.56^Ae	581.26 ± 69.58^Ae	587.53 ± 93^Ae	593.01 ± 84.35^Ae
	4	45	751.39 ± 56.45^Bb	765.24 ± 87.59^Bb	872.02 ± 61.27^ABb	870.04 ± 73.48^ABb	890.97 ± 74.44^Ab	914.59 ± 83.68^Ab	930.09 ± 107.57^Ab	943.68 ± 99.30^Ab
	25	45	564.93 ± 72.43^Bc	578.35 ± 88.22^Bc	688.16 ± 53.87^Ac	681.71 ± 66.25^Ac	698.23 ± 66.28^Ac	706.15 ± 74.9^Ac	715.67 ± 97.42^Ac	723.89 ± 89.91^Ac
	4	90	851.39 ± 71.34^Ba	881.45 ± 87.59^Ba	989.9 ± 67.6^ABa	971.2 ± 77.69^Ba	994.96 ± 76.93^ABa	1006.03 ± 87.62^Aa	1025.35 ± 110.12^Aa	1042.04 ± 103.61^Aa
	25	90	733.21 ± 76.24^Bb	745.23 ± 73.64^Bb	845.23 ± 60.01^ABb	851.66 ± 72.07^Ab	871.95 ± 74.52^Ab	882.18 ± 82.32^Ab	897.03 ± 104.9^Ab	909.85 ± 97.88^Ab
Firmness (N)	4	1	4.85 ± 0.31^Bb	4.89 ± 0.61^Bb	4.93 ± 0.37^Bab	4.96 ± 0.5^Bab	5.08 ± 0.51^Ba	5.23 ± 0.53^Bb	5.30 ± 0.79^Bb	6.62 ± 0.88^Ac
	25	1	4.28 ± 0.12^Bb	4.34 ± 0.49^Bc	4.43 ± 0.36^Bb	4.40 ± 0.49^Bb	4.5 ± 0.48^Bb	4.64 ± 0.51^Bc	4.69 ± 0.76^Bc	5.88 ± 0.84^Ad
	4	45	5.63 ± 0.27^Ba	5.75 ± 0.67^Ba	5.82 ± 0.37^Ba	5.73 ± 0.49^Ba	5.86 ± 0.47^Ba	5.96 ± 0.48^Ba	6.06 ± 0.74^Ba	9.25 ± 0.99^Ab
	25	45	4.39 ± 0.43^Bb	4.49 ± 0.7^Bc	4.61 ± 0.32^Bb	4.49 ± 0.44^Bb	4.63 ± 0.41^Bb	4.68 ± 0.42^Bc	4.74 ± 0.67^Bc	7.02 ± 0.92^Ac
	4	90	5.59 ± 0.36^Ba	5.85 ± 0.61^Ba	6.01 ± 0.37^Ba	5.83 ± 0.47^Ba	5.93 ± 0.42^Ba	6.05 ± 0.44^Ba	6.19 ± 0.69^Ba	10.14 ± 1.04^Aa
	25	90	4.95 ± 0.47^Bb	5.07 ± 0.5^Bb	5.05 ± 0.31^Bb	5.03 ± 0.42^Ba	5.19 ± 0.42^Ba	5.23 ± 0.4^Bb	5.33 ± 0.66^Bb	8.79 ± 0.98^Ab
Cohesiveness (N)	4	1	0.53 ± 0.04^Aa	0.53 ± 0.06^Aa	0.54 ± 0.04^Aa	0.54 ± 0.06^Aa	0.55 ± 0.06^Aa	0.57 ± 0.06^Aa	0.59 ± 0.09^Aa	0.66 ± 0.09^Aa
	25	1	0.49 ± 0.02^Aa	0.49 ± 0.05^Aa	0.50 ± 0.04^Aa	0.5 ± 0.05^Aa	0.51 ± 0.05^Aa	0.53 ± 0.06^Aa	0.56 ± 0.09^Aa	0.59 ± 0.08^Aa
	4	45	0.61 ± 0.03^Aa	0.62 ± 0.07^Aa	0.63 ± 0.04^Aa	0.62 ± 0.05^Aa	0.63 ± 0.05^Aa	0.64 ± 0.05^Aa	0.69 ± 0.08^Aa	0.63 ± 0.1^Aa
	25	45	0.50 ± 0.05^Aa	0.51 ± 0.07^Aa	0.52 ± 0.04^Aa	0.51 ± 0.05^Aa	0.52 ± 0.05^Aa	0.53 ± 0.05^Aa	0.58 ± 0.08^Aa	0.7 ± 0.09^Aa
	4	90	0.61 ± 0.04^Aa	0.64 ± 0.06^Aa	0.65 ± 0.04^Aa	0.63 ± 0.05^Aa	0.64 ± 0.05^Aa	0.66 ± 0.05^Aa	0.70 ± 0.08^Aa	0.98 ± 0.1^Aa
	25	90	0.56 ± 0.05^Aa	0.58 ± 0.05^Aa	0.57 ± 0.04^Aa	0.57 ± 0.05^Aa	0.59 ± 0.05^Aa	0.59 ± 0.05^Aa	0.65 ± 0.08^Aa	0.88 ± 0.1^Aa
Chewiness (N)	4	1	0.73 ± 0.05^Aa	0.72 ± 0.08^Aa	0.74 ± 0.06^Aa	0.74 ± 0.08^Aa	0.75 ± 0.08^Aa	0.78 ± 0.08^Aa	0.81 ± 0.13^Aa	0.85 ± 0.12^Ab
	25	1	0.73 ± 0.03^Aa	0.74 ± 0.08^Aa	0.75 ± 0.06^Aa	0.75 ± 0.07^Aa	0.76 ± 0.07^Aa	0.79 ± 0.08^Aa	0.84 ± 0.12^Aa	0.83 ± 0.12^Ab
	4	45	0.81 ± 0.05^Aa	0.82 ± 0.1^Aa	0.84 ± 0.06^Aa	0.82 ± 0.07^Aa	0.84 ± 0.07^Aa	0.85 ± 0.07^Aa	0.92 ± 0.11^Aa	0.94 ± 0.14^Aa
	25	45	0.74 ± 0.07^Aa	0.77 ± 0.09^Aa	0.78 ± 0.06^Aa	0.76 ± 0.07^Aa	0.78 ± 0.07^Aa	0.79 ± 0.07^Aa	0.86 ± 0.11^Aa	0.89 ± 0.13^Aa
	4	90	0.83 ± 0.06^Aa	0.87 ± 0.08^Aa	0.88 ± 0.06^Aa	0.86 ± 0.07^Aa	0.88 ± 0.07^Aa	0.9 ± 0.07^Aa	0.96 ± 0.11^Aa	0.98 ± 0.14^Aa
	25	90	0.80 ± 0.07^Aa	0.82 ± 0.07^Aa	0.81 ± 0.06^Aa	0.81 ± 0.07^Aa	0.84 ± 0.07^Aa	0.84 ± 0.07^Aa	0.92 ± 0.11^Aa	0.96 ± 0.14^Aa

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Textural properties

The firmness of the jam samples was dependent on the coating of L. plantarum, the total solids content, the storage period and temperature (Table 3). The highest amount of firmness (10.14 N) was found in the jam sample containing L. plantarum microencapsulated by 2% sodium alginate and 5% Arabic gum; there was no significant difference (P > 0.05) in the firmness value of the other samples. The firmness value was increased during the storage period, and the samples stored in the refrigerator had a higher firmness value than those stored at room temperature. Our results were in contrast with those reported by Rababah et al. (2014), who found no significant differences in the firmness value of cherry jam stored at 25 °C, 35 °C, and 45 °C for 15 days⁵⁸. The previous studies demonstrated that hydrocolloid compounds, including Arabic gum and sodium alginate caused firmer texture in the jam samples^59,60.

No significant difference (P > 0.05) was observed in the chewiness and cohesiveness of the various samples. In a study done by Teixeira et al. (2020), the results showed that the addition of orange peel in orange jam resulted in decreased adhesiveness and increased chewiness⁶¹. Moreover, Younis et al. (2015) showed that the addition of sweet lemon peel in jam caused firmness and chewiness increment and adhesiveness reduction⁶².

Sensory properties

The sensory properties (Fig. 5) of the jam samples depended on the storage time, the temperature conditions, and the type of inoculated probiotic bacteria (free or microencapsulated form) that was used. The score for the sensory properties of the jam samples, including taste, flavor, appearance, and overall acceptability, showed a decreasing trend during the storage period, which is similar to the results reported in a previous study⁵³. The reduction of the sensory property score of the jam samples that were stored at room temperature and contained free probiotic bacteria was significantly greater than the scores of the samples that were stored in the refrigerator that contained microencapsulated probiotics (P ≤ 0.05). The anthocyanin destruction and the Millard reaction that occurred during jam storage could result in a decrease in the sensory score. Furthermore, the rate of these reactions increases at a higher temperature⁵⁴. In general, the increment of sodium alginate and Arabic gum concentration, improved the sensory score so that the highest score for taste and overall acceptance was related to the jam sample containing L. plantarum microencapsulated by 2% sodium alginate and 5% Arabic gum so that this sample had significant difference (P ≤ 0.05) with other samples; thus, it was chosen as the most acceptable jam. There was no significant difference (P > 0.05) in the flavor and appearance score among the non-probiotic and probiotic jams. Sodium alginate and Arabic gum improve the texture of jam; therefore, they had a positive impact on the sensory score. Previous studies indicated that the sensory properties of various products containing microencapsulated probiotics were similar to or higher than the products containing free probiotics^51,52,63,64.

Conclusion

This study was the first attempt to produce probiotic rose petal jam. The microencapsulation of L. plantarum was performed with sodium alginate and Arabic gum to increase its viability during jam storage. There are no considerable differences between the physicochemical properties, cohesiveness and chewiness of non-probiotic jam and probiotic jam. However, the sensory assessment indicated that the jam sample containing microencapsulated L. plantarum with 2% sodium alginate and 5% Arabic gum had a higher taste and overall acceptance score than the other samples. Therefore, in general, it could be said that microencapsulation of L. plantarum with 2% sodium alginate and 5% Arabic gum and its inoculation into rose petal jam resulted in a probiotic product manufactured with physicochemical and textural properties that are similar to non-probiotic jam, and it had better sensory attributes. After 90 days of storage, the probiotic jam under room temperature and refrigerator conditions produced samples that contained a viable count of L. plantarum in an acceptable level (> 10⁶ CFU/g).

Supplementary Information

Supplementary Information 1.^{(175.8KB, docx)}

Supplementary Information 2.^{(456.9KB, docx)}

Supplementary Information 3.^{(496.8KB, docx)}

Acknowledgements

This study (Project Number: 9802241679) was approved by Ethics Committee of Hamadan University of Medical Sciences.

Author contributions

F.S.: Investigation, Data curation, Writing -original draft, Investigation, Methodology. A.H., Project administration, Conceptualization, Writing -original draft, Writing – review and editing. R.M.: Conceptualization, Investigation, Data curation. A.D.G.: Conceptualization, Writing -original draft, Writing – review and editing. M.T.: Investigation, Data curation. All of the authors read and approved the final manuscript.

Competing interests

The authors declare no competing interests.

Footnotes

Publisher's note

Springer Nature remains neutral with regard to jurisdictional claims in published maps and institutional affiliations.

Supplementary Information

The online version contains supplementary material available at 10.1038/s41598-022-10224-w.

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[CR43] 43.Rajabi H, Ghorbani M, Jafari SM, Mahoonak AS, Rajabzadeh G. Retention of saffron bioactive components by spray drying encapsulation using maltodextrin, gum Arabic and gelatin as wall materials. Food Hydrocoll. 2015;51:327–337. doi: 10.1016/j.foodhyd.2015.05.033. [DOI] [Google Scholar]

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[CR47] 47.Albadran HA, Chatzifragkou A, Khutoryanskiy VV, Charalampopoulos D. Stability of probiotic Lactobacillus plantarum in dry microcapsules under accelerated storage conditions. Food Res. Int. 2015;74:208–216. doi: 10.1016/j.foodres.2015.05.016. [DOI] [PubMed] [Google Scholar]

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[CR49] 49.Mesquita KS, Borges SV, Carneiro JDDS, Menezes CC, Marques GR. Quality alterations during storage of sugar-free guava jam with added prebiotics. J. Food Process. Preserv. 2013;37:806–813. doi: 10.1111/j.1745-4549.2012.00703.x. [DOI] [Google Scholar]

[CR50] 50.Aslam A, et al. Studying the influence of packaging materials and storage on the physiochemical and microbial characteristics of black plum (Syzygium cumini) jam. J. Food Process. Preserv. 2019;43:e13941. doi: 10.1111/jfpp.13941. [DOI] [Google Scholar]

[CR51] 51.Arslan-Tontul S, Erbas M, Gorgulu A. The Use of probiotic-loaded single-and double-layered microcapsules in cake production. Probiotics Antimicrob. Proteins. 2019;11:840–849. doi: 10.1007/s12602-018-9467-y. [DOI] [PubMed] [Google Scholar]

[CR52] 52.Mokhtari S, Jafari SM, Khomeiri M. Survival of encapsulated probiotics in pasteurized grape juice and evaluation of their properties during storage. Food Sci. Technol. Int. 2019;25:120–129. doi: 10.1177/1082013218801113. [DOI] [PubMed] [Google Scholar]

[CR53] 53.Chauhan O, Archana B, Singh A, Raju P, Bawa A. Utilization of tender coconut pulp for jam making and its quality evaluation during storage. Food Bioprocess Technol. 2013;6:1444–1449. doi: 10.1007/s11947-012-0920-8. [DOI] [Google Scholar]

[CR54] 54.Touati N, Tarazona-Díaz MP, Aguayo E, Louaileche H. Effect of storage time and temperature on the physicochemical and sensory characteristics of commercial apricot jam. Food Chem. 2014;145:23–27. doi: 10.1016/j.foodchem.2013.08.037. [DOI] [PubMed] [Google Scholar]

[CR55] 55.de Oliveira ENA, da Costa Santos D, Gomes JP, Rocha APT, da Silva WP. Physicochemical stability of diet umbu-caja jams stored under ambient conditions. J. Food Process. Preserv. 2015;39:70–79. doi: 10.1111/jfpp.12209. [DOI] [Google Scholar]

[CR56] 56.Morris GA, Castile J, Smith A, Adams GG, Harding SE. The effect of different storage temperatures on the physical properties of pectin solutions and gels. Polym Degrad. Stab. 2010;95:2670–2673. doi: 10.1016/j.polymdegradstab.2010.07.013. [DOI] [Google Scholar]

[CR57] 57.Benmeziane F, Djermoune-Arkoub L, Boudraa A, Bellaagoune S. Physicochemical characteristics and phytochemical content of jam made from melon (Cucumis melo) Int. Food Res. 2018;25:133–141. [Google Scholar]

[CR58] 58.Rababah TM, et al. Effect of jam processing and storage on phytochemicals and physiochemical properties of cherry at different temperatures. J. Food Process. Preserv. 2014;38:247–254. doi: 10.1111/j.1745-4549.2012.00770.x. [DOI] [Google Scholar]

[CR59] 59.Tan HL, Tan TC, Easa AM. The use of selected hydrocolloids to enhance cooking quality and hardness of zero-salt noodles. Int. J. Food Sci. Technol. 2018;53:1603–1610. doi: 10.1111/ijfs.13742. [DOI] [Google Scholar]

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The assessment of microencapsulated Lactobacillus plantarum survivability in rose petal jam and the changes in physicochemical, textural and sensorial characteristics of the product during storage

Fateme Shoaei

Ali Heshmati

Reza Mahjub

Amir Daraei Garmakhany

Mehdi Taheri

Abstract

Introduction

Materials and methods

Materials

Preparation of viable cells and suspension of L. plantarum

Microencapsulation of L. plantarum

Microencapsulation efficiency

The measurement of microcapsules size

The measurement of zeta potential

Morphology of microcapsules

Measurement of moisture and AW of microcapsules

The preparation of simulated gastric and intestinal juice

Survival assay of free and microencapsulated L. Plantarum after sequential incubation in simulated gastrointestinal conditions

The preparation of probiotic rose petal jam

Figure 1.

Enumeration of L. Plantarum in jam

The assessment of physicochemical, textural and sensorial characteristics of probiotic rose petal jam

Determination of TSS

The measurement of titratable acidity

The measurement of total non-reducing sugars

The color evaluation

The evaluation of texture and viscosity

The sensory evaluation

Ethical approval

Statistical analysis

Results and discussion

Physicochemical properties of the microcapsules of L. plantarum

Microencapsulation efficiency

Table 1.

Microcapsule size and morphology

Zeta potential of microcapsules

Moisture content and AW of microcapsules

The survival of free and encapsulated L. plantarum during sequential incubation in simulated gastrointestinal conditions

Figure 2.

The survival of L. plantarum during jam storage in different conditions

Figure 3.

Effect of storage time and temperature on the physicochemical, textural and sensorial characteristics of probiotic and non-probiotic rose petal jam

pH and acidity

Figure 4.

TSS

Total non-reducing sugars

Color

Table 2.

Viscosity

Table 3.

Textural properties

Sensory properties

Figure 5.

Conclusion

Supplementary Information

Acknowledgements

Author contributions

Competing interests

Footnotes

Supplementary Information

References

Associated Data

Supplementary Materials

ACTIONS

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