Antioxidant Activity Of Lactobacillus Plantarum NJAU-01 in An Animal Model Of Aging
Sep 29, 2022
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Abstract
Background: Excessive reactive oxygen species (ROS) can cause serious damage to the human body and may cause various chronic diseases. Studies have found thatlactic acid bacteria (LAB) have antioxidant and anti-aging effects, and are important resources for the development of microbial antioxidants. This paper was to explore the potential role of an antioxidant strain, Lactobacillus plantarum NJAU-01 screened from traditional dry-cured meat product Jinhua Ham in regulating D-galactose-induceed subacute senescence of mice. A total of 48 specific pathogen free Kun Ming mice (SPF KM mice) were rancomly allocated into 6 groups: control group with sterile saline injection, aging group with subcutaneously injection of D-galactose, treatments groups with injection of D-galactose and intragastric administration of 10’,10°, and10°CFU/mL L.plantarum NJAU-01,and positive control group with injection of D-galactose and intragastric administration of 1 mg/mL Vitamin C.
Results: The results showed that the treatment group ofL. plantarum NJAU-01 at 10°CFU/mL showed higher total antioxidant capacity (T-AOC) and the antioxidant enzymatic activities of superoxide dismutase (SOD), glutathione peroxidase (GSH-Px), and catalase(CAT) than those of the other groups in serum, heart and liver. In contrast, the content of the oxidative stress marker malondialdehyde(MDA) showed lower levels than the other groups (P<0.05). The antioxidant capacity was improved with the supplement of the increasing concentration of L. plantarum NJAU-01.

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Conclusions: Thus, this study demonstrates that L plantarum NJAU-01 can alleviate oxidative stress by increasing the activities of enzymes involved in oxidation resistance and decreasing level of lipid oxidation in mice. Keywords: Lactobacillus Plantarum NJAU-01, Jinhua Halm, D-galactose-induced aging animal, Malondialdehyde, Antioxidant capacity
Background
Oxidation is a process necessarily required for cellular metabolism in the body. The reactive oxygen species (ROS) as free radicals produced by endogenous oxidation-reduction (REDOX) reactions were respon-sible for the oxidation. However, when the cells receive oxidative stress-induced external stimuli, excessive pro-duction of ROS overwhelms the cellular ROS scavenging capacity [1]. Some research data have shown that oxida-tive stress is related with the lifespan of organisms [2]Unable to metabolize the remaining ROS can cause ser-ious damage to the human body and may cause various chronic diseases related to aging, such as diabetes, heart disease, high blood lipids, arthritis, neurodegenerative diseases, cardiovascular and cerebrovascular diseases [3]. Normally, the body has a series of enzymes or non-enzymes and repair systems which are involved in antioxidant defense and protect them from oxidative damage [4-6]. For example, ascorbic acid consumes oxy-gen through self-oxidation, reducing metal ions to lower the oxidation-reduction potential and being involved in antioxidant defense [7]. Superoxide dismutase (SOD) is able to convert harmful superoxide radicals into hydro-gen peroxide [8]. Catalase (CAT) participates in cellular antioxidant defense by decomposing hydrogen peroxide, thereby preventing the Fenton reaction from producing hydroxyl free radicals [9]. However, superfluous ROS would lead to oxidative damage caused by many factors like irradiation (X-rays, y-rays, ultraviolet), chemical re-agents (metal ions, HONO, HOCl, and HOBr), drug and their metabolites, and even smoking. These natural antioxidant systems in the body are often insufficient to prevent oxidative damage, requiring antioxidants supplements such as astaxanthin and folic acid [10]. Thus, the search for available approach that can alleviate or inhibit cellular oxidative damage has received considerable attention.
Lactic acid bacteria (LAB) have been widely found and utilized in fermented meat products. Besides improving the nutrient, flavor, and preservation of fermented food, LAB also have additional probiotic characteristics [11, 12]. Some studies have found that LAB have antioxidant and anti-aging effects, and are important resources for the development of microbial antioxidants [13]. For in-stance,Lactobacillus case separated from Chinese home-made liqueur, was found to effectively alleviate lipid peroxidation and improve lipid metabolism due to high cholesterol scavenging ability and human intestinal cell adhesion ability [14]. We have previously isolated and screened a lactic acid bacteria by total antioxidant cap-acity from Jinhua ham and identified it as Lactobacillus plantarum by detecting biochemical characteristics, co-lonial morphology, and 16 s rDNA sequencing, named L. plantarum NJAU-01 [15]. L. plantarum NJAU-01 showed excellent scavenging power and reducing power of DPPH free radicals, hydroxyl free radicals, and super-oxide anion free radicals in vitro [16]. In the cell model coupled with electrochemical sensor, the ability of macrophage RAW264.7 in response to oxidative stress was significantly enhanced by incubation with L. plan-tarum NJAU-01 [15]. Cistanche Extract Anti Radiation In addition,L. plantarum NJAU-01 could also alleviate the degree of protein oxidation in fermented sausage [17]. Thus,L. plantarum NJAU-01 has been proved to have an antioxidant effect in vitro, which is promising to be potentially utilized in regulat-ing oxidative stress in vivo.

Cistanche can anti-aging
Thus it is essential to assess the antioxidant effect of L. Plantarum NJAU-01 in vivo by using the animal model, which can effectively observe the absorption, transporta-tion and metabolism in animals. D-galactose-induced aging mice have been developed to simulate the occurrence of oxidative damage in the aging process of the body for decades [18]. D-galactose contributes to the generation of ROS via reaction with amino acids to form glycation end products through non-enzymatic glycation with the benefits of low toxicity, slow oxidation process, and no lethal effect [19,20]. D-galactose-induced aging mice model has often been reported to evaluate the anti-oxidant capacity of probiotics such as L-carnitine, ursolic acid and L. Plantarum AR501 [19,21,22]. Therefore, these mature D-galactose-induced aging mice were used for preliminary investigation of the role of L. plantarum NJAU-01 in relieving oxidative stress in mice. L. plan-tarum NJAU-01 was fed to D-galactose-induced aging mice to evaluate its in vivo antioxidant effects by measuring the total antioxidant capacity (T-AOC), the anti-oxidant enzymatic activities of SOD, glutathione peroxidase (GSH-Px), and CAT, as well as the content of the oxidative stress marker malondialdehyde (MDA)in mice serum, heart and liver. cistanche herba This will provide the basis for further research on the development and utilization of L. plantarum NJAU-01 as a probiotic.
Results
Body weight and organ indices in mice
None of the animals died during the feeding period and date from all mice were included. The effects of different treatments with L. plantarum NJAU-01 on the organ in-dices of mice are shown in Table 1. The mice in aging group injected with D-galactose showed significantly lower body weight compared with that of the other groups (P<0.05). no="" significant="" difference="" was="" ob-served="" in="" kidney="" liver="" index="" and="" lung="" be-tween="" the="" l.="" plantarum="" njau-01="" treatment="" groups="" normal="" positive="" group="" aging="" model="" p="">0.05). The heart index of the aging model group was significantly higher compared to that of the normal group (P<0.05).
T-AOC activity of serum, heart, and liver of mice The T-AOC activity of mice among different treatment groups is shown in Fig. 1. The T-AOC activity of the aging mice model group was 6.68 U/mL, and while in heart, serum and liver were 6.62,3.55 and 3.58 U/mg protein, respectively, which were lower than other groups (P<0.05). In the L. plantarum NJAU-01 LP3 group, serum, heart, and liver had significantly higher T-AOC than the other groups (P<0.05). The liver T-AOC in the positive control group was significantly higher than the control group and the aging model group (P<0.05). However, the antioxidant activity of the heart and liver of the positive control group was significantly lower than that of the LP3 group (P<0.05). The above results indicate that L. Plantarum NJAU-01 can enhance the T-AOC of the mice in a dose-dependent manner.

SOD activity in mice serum, heart, and liver
The SOD activities of mice in the aging model group in serum, heart and liver of mice were 16.72 U/mL,18.93 U/mg protein and 44.82 U/mg protein respectively, which were significantly lower than the control group (P<0.05,Fig.2).In contrast,the SOD activity in serum, heart and liver of mice in Vc group was significantly higher than that of mice in the aging model group and control group (P<0.05). the="" sod="" activity="" in="" heart="" of="" mice="" lp2="" group="" was="" 61.85="" mg="" which="" not="" significantly="" different="" from="" that="" positive="" control="" p="">0.05). On the other hand, the SOD activities in the serum, heart and liver of high dose group were 48.83 U/mL,74.67 U/mg protein and 69.55 U/mg protein respectively, which were significantly higher than that in the other groups (P<0.05). These results showed that L. Plantarum NJAU-01 could alleviate the oxidative damage induced by D-galactose to the body, and increase SOD activity.
GSH-Px in mice serum, heart, and liver
LP3 group presented higher GSH-PX activity than that of mice in other groups in serum, heart and liver (P<0.05, Fig. 3). The GSH-Px activity in the heart and liver tissues of mice in the positive control group was signifi-cantly higher than that of mice in the control group and the aging model group (P<0.05). there="" was="" no="" significant="" difference="" for="" the="" serum="" gsh-px="" activity="" between="" lp1="" and="" control="" group="" p="">0.05).In addition, the aging model groups in the heart and liver of mice were 50.39 U/mL,8.48 U/mg protein and 62.67 U/mg protein respectively, showing lower GSH-Px activity than the other groups (P<0.05). Therefore,L. plantarum NJAU-01 has an enhancing effect on the antioxidant enzymatic activity of GSH-Px in mice, and the strain concentration is related to the antioxidant effect.
CAT activity in mice serum, heart and liver
As shown in Fig. 4, the CAT activities of serum, heart and liver of LP3 mice were 22.98 U/mL,137.99 U/mg protein and 136.31 U/mg protein respectively, which possessed higher CAT activity than that in other treat-ment groups (P<0.05), indicating that the concentration of the strain had a marked effect on the CAT activity. cistanche penis growth In contrast, the aging model group showed lower CAT ac-tivity than that of mice in the other groups in serum, heart and liver of mice (P<0.05). As for Vc group, it presented higher CAT activity than the control group and aging model group in serum, heart and liver of mice (P<0.05). These findings demonstrate that L. Plantarum NJAU-01 can enhance the CAT activity in mice serum, heart and liver tissues.
MDA content in mice serum, heart and liver
MDA content in serum, heart and liver of mice in the aging model group was significantly higher than the con-trol group (P<0.05, Fig. 5). The serum MDA content of mice in the LP3 group was 14.29 nmol/mL, and the MDA contents in the heart and liver were 8.00 and 26.49 nmol/mg protein, respectively, being significantly lower than that in the other groups (P<0.05). there="" was="" no="" significant="" difference="" in="" mda="" content="" among="" the="" positive="" control="" lp1="" and="" lp2="" groups="" p="">0.05).
Discussion
The subacute aging mice model by the D-galactose in-duction is widely used and well-recognized [14,23,24]. The model involves continuous injection of D-galactose which is reduced to galactose by galactose reductase in-side the cells, resulting in change of osmotic pressure between the cell and the environment and then cell swelling and aging [25]. Intracellular enzymes that re-lieve oxidative stress, such as SOD, CAT and GSH-Px, are not sufficient to eliminate reactive oxygen species, when the cells in the body are subjected to acute oxida-tive stress. It is a direct and effective method to study the antioxidant activity of LAB by injecting LAB into D-galactose-induced subacute aging mice and comparing enzymatic antioxidant activity, such as SOD, GSH-Px, and CAT with the control group [21].

In this study, the aging model group and the positive control (injection with Vc) group were compared with different doses of the L. plantarum NJAU-01 treatment group. The organ index is the ratio of the weight of an organ in the experimental animal to its body weight and an increase in the organ coefficient indicates congestion, edema, or hyperplasia of the organ while a decrease in the organ coefficient indicates organ atrophy and other degenerative changes. The organ index was also used to express the changes in degree of aging as evidenced in studies of Yu et al. (2016) and Xu et al. (2016)[18,26]. The present study revealed that the mice in aging model group had lower weight and higher heart index than that of mice in the other groups. The administration of D-galactose significantly decreased the antioxidant en-zymatic activity in serum, heart and liver of mice in the aging model group. The L. plantarum NJAU-01 supple-ments was suggested to reduce the liver injury of D-galactose-induced oxidative stress mice by regulating abnormal activities of SOD, GSH-Px, and CAT to nor-mal levels. It is in accord with the reported studies when investigating the antioxidant role the targeted strains including L. plantarum AR113 and ARS01 [12],L. del-brueckii subsp. bulgaricus F17 [27]. Thus, D-galactose subacute mice model of aging in the current study is ef-ficient to provide confidential evidence for investi-gating the antioxidant capacity of LAB in vivo.
Previous research results have indicated that the anti-oxidant mechanism of LAB is mainly manifested in the following aspects: chelated metal ions, autotrophic anti-oxidant enzyme systems, production of antioxidant me-tabolites, increased host antioxidant enzyme activity, control of antioxidant signaling pathways, and regulation of intestinal bacteria group [28]. These aspects play a critical role in alleviating diseases whose development involves with oxidative stress [29]. MDA is considered as the biomarker of lipid peroxidation, and it can lead to cross-linked polymerization of macromolecules, playing a potential role in cytotoxicity and genotoxicity. The content of MDA is usually used as a basis for evaluating the degree of lipid peroxidation and reflecting the level of damage to cells [30]. cistanche salsa benefits The current study found that mice with D-galactose-induced oxidative stress had sig-nificantly reduced MDA levels in serum, heart and liver by injecting with L. plantarum NJAU-01 indicating that L. Plantarum may effectively reduce the formation of lipid peroxide in mice. This is consistent with in vitro study, which showed effective free radical scavenging ability of the L. plantarum NJAU-01 strain [16]. Simi-larly, weaned piglets fed with L. plantarum ZLP001 presented a lower serum MDA content (4.1 nmol/ml) than the control group (6.23 nmol/ml), demonstrating that L. Plantarum ZLP001 possessed antioxidant activity [31]. The current study suggested that L. plantarum NJAU-01 supplements could essentially relieve the degree of lipid oxidation in D-galactose-induced mice, protecting the mice from oxidative stress.
There is a set of free radical scavenging enzyme defense systems in the body, such as SOD, GSH-Px and CAT, which synergistically scavenge superoxide radicals, hy-droxyl radicals and hydrogen peroxide, respectively [32]The free radical oxidation and the antioxidant defense system of the organism are in a state of dynamic equilib-rium. When the body is exposed to oxidative stress inducing stimuli, this dynamic balance might be disrupted. Excessive production of ROS damages proteins, lipids and nucleic acid molecules, ultimately leading to the aging of organisms and the development of various diseases [3]. SOD can convert superoxide radicals to hydrogen perox-ide, which is still cytotoxic and can generate hydroxyl radi-cals by Fenton reaction [34]. Hydroxyl radical is one of the most active ROS, which can react with organic matter in the cell with the fast reaction rate and destructive effect [35]. Moreover, CAT can decompose hydroxyl radicals to participate in cell antioxidant defense [36]. Under physiological conditions, antioxidant enzymes, such as GSH-Px can be produced in cells to protect these cells from oxida-tive damage [25]. This study showed that L. plantarum NJAU-01 can significantly enhance the activities of SOD, GSH-Px, CAT and T-AOC in serum, heart and liver of mice, indicating that L. plantarum NJAU-01 alleviates the oxidative damage caused by D-galactose. This effect may be attributed to two aspects.L. plantarum NAJU-01 can promote the activity of antioxidant enzymes in mice, regulating the equilibrium of ROS to normal levels in mice. On the other hand, it also could scavenge free radicals and act synergistically with SOD, GSH-Px and CAT to reduce oxidative stress. Regulation of activities of antioxidant enzymes by the probiotic bacteria was also reported for Lactobacillus fermentum [37] and Lactobacillus fermen-tum ME-3 [38]. This study demonstrates that L. plan-tarum NJAU-01 exerts an antioxidant effect in mice and is a promising alternative to synthetic or plant-derived antioxidants. It is usually used as a bio-source antioxidant for the study of sausage starters or functional products [18]. Although research on the antioxidant activity of LAB has achieved wide attention in recent years, investigations on the underlying mechanism of L. Plantarum NJAU-01 anti-oxidation, in particular, the metabolic pathways, the protein expression and the regulation of intestinal flora are still scant. Moreover, the cross and complementation of multiple antioxidant mechanisms in lactic acid bacteria require further investigation.
Conclusions
This preliminary study evidenced the effect of L. plan-term NJAU-01 isolated from Jinhua ham on the D-galactose-induced aging model of mice. It was found that the addition of L. Plantarum NJAU-01 during the feeding process of mice can significantly increase the activity of antioxidant enzymes and decrease the content of MDA. This study confirms the possibility of L. plan-tarum NJAU-01 as a bio-antioxidant and lays the foundation for further study of the antioxidant mechanism of L.plantarum.
Methods
Bacterial strain and animal preparation
L.plantarum NJAU-01 (CGMCC14194) was screened from the traditionally dry-cured meat product Jinhua ham using morphological, biochemical and molecular genetic identification methods [15]. This strain had high antioxidant activity and was preserved in the College of Food Science and Engineering of Yangzhou University [16]. Lactobacillus Plantarum NJAU-01 was preserved as frozen (-80 ℃) stocks in De Man, Rogosa, Sharpe (MRS) broth(Bio-way Technology Co., Ltd, Shanghai, China) supplemented with 20% (v/v) glycerol. The strain of 1% inoculum was activated twice and grown in 10 mL MRS broth at 37℃ for 18h. The bacterial suspension of 100 μL was then inoculated into the solid MRS medium by the automatic diluter and plater (Reference 414,000, Interscience, Saint-Nom-la-Breteche, France). The inoculated MRS solid medium was cultured at 37°C for 24 h, and the viable count was counted by the automatic HD colony counter (Scan 1200, Interscience, Saint-Nom-la-Breteche, France) and Scan° software version 8.0 (Interscience, Saint-Nom-la-Breteche, France). The concentration of bacterial suspension was detected to be 2×10' CFU/mL, and the strain culture of 10 mL was centrifuged at 6,000 g for 10 min at 4 ℃ to discard the supernatant. The pellet was washed with sterile saline for three times and then dissolved in 20 mL of sterile saline, obtaining 1×10°CFU/mL of L.plantarum NJAU-01. Then, an aliquot of 2 mL bacterial suspension at 1×10°CFU/mL was removed into a new tube to combine with 18 mL of sterile saline for making a dose of 1×10°CFU/mL bacteria. Analogically, the concentration of 1×107 CFU/mL was made by the dilution of 1×10°CFU/mL bacterial suspension. The SPF grade KM mice (female, 4 weeks old, weighing 18-20 g) were chosen for the experimental animal. Animal feed and bedding were provided by the Institute of Comparative Medicine of Yangzhou University (Yangzhou, Jiangsu, China). All animal experiments were approved by the Animal Welfare and Ethics Committees of Yangzhou University and complied with the guidelines of the Institutional Administrative Committee and Ethics Committee of Laboratory Animals (IACUC license number:201811009). The mice were raised at 20±2℃ with a relative humidity of 55±5%. The rats were randomly fed a standard rat diet during a half-day light and dark cycle (light phase from 7:00 am to 7:00 pm). Four mice were raised in a cage, fed with a pathogen-free diet and water. All materials, including lids, feeders, bottles, and bedding were autoclaved before use. The mice were acclimated for one week before the establishment of mice aging model.
Establishment of mice model of aging
The subacute D-galactose-induced mice model of aging was established and referred to Zhao et al. with slight modifications [39]. The galactose administration method was conducted by subcutaneous injection in the neck and back. A total of 48 SPF mice were randomly assigned into 6 groups(8 rats/group)after one week of acclimation. Random numbers were generated using the standard=RAND() function in Microsoft Excel. Mice in every group, except the control group, were subcutaneously injected with 500 mg D-galactose per kg body weight (Shanghai Blue Season Biological Co.,Ltd, Shanghai, China) for 4 weeks once a day (D-galactose solution, 50 g/L). The control group was injected with 10 mL sterile saline per kg body weight. In addition, the three treatment groups were given intragastric doses of L. cistanche tubulosa dosage reddit Plantarum NJAU-01 (10' CFU/mL, 10° CFU/mL, and 10°CFU/mL) at 20 mL per kg body weight, and designated as LP1 group,LP2 group and LP3 group, respectively. The mice in control group and the aging group were intragastrically fed with sterile saline at 20 mL/kg daily. The mice in the positive control group were treated with 1 mg/mL vitamin C (Vc) at 20 mL/kg daily. The entire experiment lasted four weeks.
Preparation of tissue samples
Mice were euthanized to an unconscious state by intraperitoneal injection of 3% isoflurane. Cessation of heart-beats and non-responsiveness to noxious stimulus (hind paw pinch) were used as criteria to verify death. The eyeball of the mice was removed, and blood was drawn. Then, the blood was immediately centrifuged at 3,00xg for 10 min at 4℃ to obtain the serum and stored at -20℃ until analyzed. After being euthanized, the mice were executed unconsciously by pulling cervical verte-brae, and liver, heart, spleen, kidney,lung and brain were harvested, and weighed to determine the organ indices. The liver and heart samples were homogenized into 10% tissue homogenate with 0.9% NaCl, and the super-natant was collected by centrifugation as above-mentioned.
Parameter detections
The T-AOC and the antioxidant enzymatic activities of SOD, GSH-Px, and CAT, and the contents of MDA were determined using total antioxidant capacity assay kit (ABTS method, A015-2-1), superoxide dismutase (SOD) assay kit (WST-1 method, A001-1-2), glutathione peroxidase (GSH-PX) assay kit (Colorimetric method, A0060201), catalase (CAT) assay kit (Colorimetric method, A007-2-1) and malondialdehyde (MDA) assay kit (TBA method, A003-2-1), respectively. All kits were purchased from Nanjing Jiancheng Bioengineering Institute Co, Ltd (Nanjing, Jiangsu, China). All samples were tested in triplicate, and the detection procedures were conducted in accordance with the instructions.
Statistical analysis
The data were analyzed using the Data Processing System 7.05 software (Hangzhou Ruifeng Information Technology Co., Ltd, Hangzhou, China). Different of means was compared by the Duncan's new complex range method. The statistical significance test was performed at the 0.05 level (P<0.05).
This article is extracted from Ge et al. BMC Microbiology (2021) 21:182 https://doi.org/10.1186/s12866-021-02248-5






