TQ (HPLC ≥99%, CAS 490-91-5) was purchased from Aladdin Biochemical Technology Co., Ltd (Shanghai, China). The commercial compound was dissolved in dimethyl sulfoxide (DMSO) and diluted with sterile deionized water or A. acidoterrestris medium (AAM, 2.0 g of glucose, 2.0 g of yeast extract, 1.0 g of magnesium sulfate, 1.2 g of potassium dihydrogen phosphate, 0.2 g of ammonium sulfate, and 0.25 g of calcium chloride per liter of distilled water) before use. The final concentration of DMSO in all sample solutions was 1% (v/v). All other chemicals and reagents were of analytical grade.

The DSM 3922, DSM 3923, and DSM 2498 strains of A. acidoterrestris were purchased from the German Resource Centre for Biological Material (DSMZ). Two other A. acidoterrestris isolates (GYL-02, GYL-11) were obtained from our laboratory strain collection, and originated from the fruit granary of Shaanxi province. Minimum inhibitory concentrations (MICs) determination experiments were conducted for all five A. acidoterrestris strains; however, only DSM 3922 was used in subsequent assays. The strains were stored in AAM broth containing 25% (v/v) glycerol at −80°C before use. A. acidoterrestris working suspensions were prepared as follows: First, stock cultures were inoculated onto AAM plates and incubated at 45°C for 24 h. Then, the bacterial colony was transferred to AAM broth and incubated at 45°C for 12 h with shaking at 120 rpm. Next, the bacterial suspensions were centrifuged (4,000 × g, 5 min, 4°C), washed twice with phosphate buffered saline (PBS), and resuspended in sterile AAM broth. Then the optical density of the suspension at 600 nm (OD_{600 nm}) was adjusted to 0.5 for use.

To prepare spore suspension, the methods described by Cai et al. (2019b) and Prado et al. (2019) were followed with some modifications. A. acidoterrestris vegetative cells were cultured in AAM broth at 45°C for 15 days until about 90% sporulation was observed under a phase contrast microscopy. Subsequently, the cell culture was centrifuged (4,000 × g, 10 min, 4°C), washed twice, and resuspended in cold sterile saline. The spore concentration of the suspension was determined by heat shock (80°C for 10 min), serial dilution, and plating on AAM agar, which proved to be ∼10⁶ spores/mL. Finally, the suspension was stored at 4°C until use.

The MICs of TQ against five A. acidoterrestris strains were measured using a modified version of the broth dilution method, based on the guidelines of the Clinical and Laboratory Standards Institute (Clinical and Laboratory Standards Institute (CLSI), 2009). A. acidoterrestris suspensions (OD_{600 nm} ≈ 0.5) were diluted in AAM broth to achieve the working suspension with a cell concentration of ∼10⁵ CFU/mL. Subsequently, the suspension was transferred to a 96-well plate, followed by the addition of TQ solutions. The final concentrations of TQ were 0 (control), 8, 16, 32, 64, 128, 256, and 512 μg/mL, respectively. AAM broth containing 1% DMSO but no TQ was taken as negative control. The plates were incubated at 45°C for 24 h, and the lowest concentration at which no visible bacterial growth was observed was considered as the MIC of TQ.

A. acidoterrestris DSM 3922 suspensions with an OD_{600 nm} of 0.2 (∼3 × 10⁴ CFU/mL) were inoculated into the wells of a 96-well plate. TQ was added into the corresponding wells to obtain the final concentrations of 0 (control), 1/16 × MIC, 1/8 × MIC, 1/4 × MIC, 1/2 × MIC, and 1 × MIC, respectively. Then the plate was incubated at 45°C for 24 h and the OD_{600 nm} values were measured by a multimode plate reader (Tecan, Infinite^TM M200 PRO, Mannedorf, Switzerland), at 2-h intervals in order to monitor the growth of A. acidoterrestris cells.

To assess the bactericidal activity of TQ against A. acidoterrestris, the time-kill assay was performed as described by Shi et al. (2016). A. acidoterrestris DSM 3922 suspensions were diluted in AAM broth to a cell concentration of ∼10⁵ CFU/mL. TQ was added to the suspensions to achieve final concentrations of 0 (control), 1/2 × MIC, 1 × MIC, and 2 × MIC, respectively. Then the samples were incubated at 45°C for 0, 3, 6, 9, 12, or 24 h. At each time point, samples were diluted in sterile PBS and spread onto AAM agar for viable enumeration.

Following the method of Kang et al. (2019), FESEM observation was conducted with slight modifications. Briefly, A. acidoterrestris cells treated with TQ (0, 1 × MIC, and 2 × MIC) were incubated at 45°C for 2 h, followed by centrifugation (3,000 × g, 5 min, 4°C) and washing twice with PBS. The A. acidoterrestris cells were fixed with 2.5% glutaraldehyde at 4°C for 12 h and dehydrated with 30, 50, 70, 80, 90, and 100% water-ethanol solutions for 10 min, respectively. After critical point drying and gold spray treatment, samples were observed using a field-emission scanning electron microscope (Nano SEM-450, FEI, United States).

CLSM observation was carried out according to the method described by Song et al. (2019), with minor modifications. A. acidoterrestris DSM 3922 suspensions treated with TQ (0, 1 × MIC, and 2 × MIC) were incubated at 45°C for 60 min. Then the suspensions were centrifuged (3,000 × g, 5 min, 4°C) and resuspended with 0.85% sterile saline. Following the addition of propidium iodide (PI) and SYTO 9, the suspensions were incubated in the dark for 15 min. Finally, the samples were deposited on a glass slide for CLSM analysis at the excitation/emission wavelengths of 480/500 nm (SYTO 9) and 490/635 nm (PI).

With slight modifications, the method of Prado et al. (2019) was used in this assay. Briefly, A. acidoterrestris spore suspensions (stored at 4°C for about 1 month) were diluted with 0.85% sterile saline to achieve a cell density of 10⁴ ∼ 10⁵ CFU/mL. TQ was then added to obtain final concentrations of 0 (control), 4 × MIC, 8 × MIC, and 16 × MIC, respectively. The spores in the control group were not treated with TQ. Then samples were incubated at 45°C for 0, 30, 60, 120, 180, 240, or 360 min. At each time point, samples were taken, diluted, and spread onto AAM agar, followed by incubation and viable counts.

To confirm the inactivation effect of TQ on spores, the morphology of TQ-treated spores was observed using FESEM. The spore suspensions mentioned above were treated with TQ (0, 4 × MIC, 8 × MIC, and 16 × MIC) at 45°C for 6 h. Samples were centrifuged at 4,000 × g at 4°C for 10 min and the cells were fixed with 2.5% glutaraldehyde. The following gradient dehydration, critical point drying, gold spray treatment, and FESEM observations were the same as described in above section.

With minor modifications, the method described by Fan et al. (2018) was followed. A. acidoterrestris DSM 3922 suspensions were co-incubated with sterile stainless steel sheets (5 mm × 5 mm) in a sterile 24-well flat-bottomed plate at 45°C for 24 h. The sheets were gently rinsed with PBS and carefully transferred to the new wells containing TQ solutions at 0 (control), 2 × MIC, 4 × MIC, and 8 × MIC. After an incubation at 45°C for 4 h, the sheets were washed gently with PBS before being immersed in a 2.5% glutaraldehyde solution for fixing. The following gradient dehydration, critical point drying, gold spray treatment, and FESEM analysis were conducted as described in the above section.

The IBM SPSS software (New York, United States) was used for statistical analysis. All experiments were performed three times, and the data were expressed as mean ± standard deviation. The differences between means were tested by two-way analysis of variance and were considered significant at p < 0.05.

As shown in Table 1, the MICs of TQ against five A. acidoterrestris strains ranged from 32 to 64 μg/mL. The results suggested that TQ was effective at inhibiting A. acidoterrestris and may be used as a potential method to control A. acidoterrestris in the food industry.

The effect of TQ on the growth of A. acidoterrestris DSM 3922 is presented in Figure 1A. In the presence of TQ (1 × MIC), the OD_{600 nm} of the A. acidoterrestris suspension remained steady within 24 h, suggesting that this concentration of TQ inhibited the growth of A. acidoterrestris. In the presence of TQ (1/4 × MIC, 1/8 × MIC, and 1/16 × MIC), the OD_{600 nm} of the A. acidoterrestris suspension increased continuously over time, indicating that TQ at these concentrations could not inhibit the bacterial growth.

The bactericidal effect of TQ on A. acidoterrestris DSM 3922 is shown in Figure 1B. The initial number of A. acidoterrestris cells in the samples was 4.8 log CFU/mL. Viable cells counts in the group treated with TQ (1/2 × MIC) decreased to 4.4 log CFU/mL and then increased continually to 7.1 log CFU/mL. In contrast, the number of cells in groups exposed to TQ (1 × MIC and 2 × MIC) reduced constantly over time. At 3 h post-treatment, TQ at 1 × MIC and 2 × MIC reduced the cell counts to 3.5 and 2.6 log CFU/mL, respectively. And at 24 h post-treatment, TQ at the two concentrations caused greater reductions to 2.9 and 1.8 log CFU/mL, respectively. The results revealed that TQ at 1 × MIC and 2 × MIC exerted a bactericidal effect on A. acidoterrestris cells.

The changes in A. acidoterrestris cell morphology caused by TQ were confirmed by FESEM observation. As shown in Figure 2, untreated A. acidoterrestris cells were regular, smooth, plump, and rod-shaped. Whereas after exposure to TQ (1 × MIC and 2 × MIC) for 2 h, the surfaces of the A. acidoterrestris cells became rough, irregular, and wrinkled. Moreover, perforations and cankers were observed. The results revealed that TQ at 1 × MIC and 2 × MIC destroyed the cell morphology of A. acidoterrestris.

The damage of TQ to A. acidoterrestris membrane integrity was assessed using fluorescent dyes SYTO 9 and PI by CLSM observation. SYTO 9 is a nucleic acid dye which can penetrate all bacterial cells, combine with DNA, and generate green fluorescence. By contrast, PI only stains the bacterial cells that have a damaged cell membrane and it generates red fluorescence. As presented in Figure 3, A. acidoterrestris cells in the control group exhibited complete green fluorescence and almost no red fluorescence was observed, suggesting that cells in this group had an intact membrane. In contrast, a small amount of red fluorescence occurred after treatment with TQ at 1 × MIC, indicating that the membrane integrity of some cells was destroyed by TQ. After exposure to TQ at 2 × MIC, a dramatic increase in red fluorescence intensity was observed, showing that this concentration of TQ resulted in a more damaged cell membrane. Overall, these findings demonstrated that TQ could impair the cell membrane of A. acidoterrestris in a dose-dependent manner.

The killing effect of TQ (0, 4 × MIC, 8 × MIC, and 16 × MIC) on A. acidoterrestris spores is shown in Figure 4. The number of spores at 0 min in all samples were 4.7 log CFU/mL. Obviously, the number of spores in the untreated group remained the same throughout the experiment, while the number of spores in the TQ-treated groups decreased over time. At 240 min post-treatment, TQ (4 × MIC, 8 × MIC, and 16 × MIC) reduced the spore counts to 4.4, 4.0, and 3.8 log CFU/mL, respectively. And greater reductions to 4.2, 3.8, and 3.5 log CFU/mL were achieved at 360 min post-treatment. The results revealed that TQ exerted a moderate inactivation effect on A. acidoterrestris spores.

The effect of TQ on A. acidoterrestris spores was further verified by FESEM observation. As presented in Figure 5, untreated spores exhibited a normal morphology with an oval, smooth, and plump shape. After exposure to TQ (4 × MIC) for 6 h, the surface of spores became rough, wrinkled, or even hollow. Moreover, rupturing and cracks occurred on the surface as the concentration of TQ increased to 8 × MIC and 16 × MIC.

The inactivation effects of TQ on A. acidoterrestris biofilms formed on polystyrene and stainless steel surfaces are shown in Figures 6A,B. Obviously, TQ treatments reduced the number of viable cells in biofilms formed on the two surfaces. The initial number of A. acidoterrestris cells on biofilms formed on the polystyrene surface was 5.5 log CFU/ml and decreased to 4.9, 3.8, 3.0 log CFU/ml, 4.8, 3.4, 2.6 log CFU/ml, and 4.6, 2.9, 1.9 log CFU/ml after treatment with TQ (2 × MIC, 4 × MIC, 8 × MIC) for 60, 120, and 180 min, respectively. Similarly, TQ reduced the number of A. acidoterrestris cells in biofilms formed on the stainless steel surface. At the initiation of treatment, the total number of viable A. acidoterrestris cells on stainless steel surfaces was 5.9 log CFU/ml. Whereas at 60, 120, and 180 min post-treatment of TQ (2 × MIC, 4 × MIC, 8 × MIC), viable counts in the biofilms were reduced to 5.6, 5.1, 4.5 log CFU/ml, 5.0, 4.4, 3.8 log CFU/ml, and 4.7, 3.9, 3.2 log CFU/ml, respectively. The results indicated that TQ could inactivate A. acidoterrestris cells on biofilms developed on polystyrene and stainless steel surfaces in a concentration-dependent manner.

The elimination effect of TQ on A. acidoterrestris biofilms was confirmed by FESEM observation and the images are presented in Figure 7. A. acidoterrestris biofilms in the control group were dense, evenly distributed, and had a multilayer structure with clustered cells. Nevertheless, at 4 h post-treatment of TQ (2 × MIC and 4 × MIC), the layer became thin, uneven, and the cell clusters in the biofilm decreased. After treatment with TQ at 8 × MIC, the number of A. acidoterrestris cells adhered to the surface decreased significantly and no A. acidoterrestris clusters were observed. The results suggested that TQ may be applied as an antibiofilm agent in the food industry to control A. acidoterrestris biofilms.