Pseudomonas species prevalence, protein analysis, and antibiotic resistance: an evolving public health challenge

Psychrotrophic Pseudomonas is one of the significant microbes that lead to putrefaction in chilled meat. One of the biggest problems in the detection of Pseudomonas is that several species are seemingly identical. Currently, antibiotic resistance is one of the most significant challenges facing the world's health and food security. Therefore, this study was designed to apply an accurate technique for eliminating the identification discrepancy of Pseudomonas species and to study their resistance against various antimicrobials. A total of 320 chicken meat specimens were cultivated, and the isolated bacteria’ were phenotypically recognized. Protein analysis was carried out for cultured isolates via Microflex LT. The resistance of Pseudomonas isolates was recorded through Vitek® 2 AST-GN83 cards. Overall, 69 samples were identified as Pseudomonas spp. and included 18 Pseudomonas lundensis (P. lundensis), 16 Pseudomonas fragi (P. fragi), 13 Pseudomonas oryzihabitans (P. oryzihabitans), 10 Pseudomonas stutzeri (P. stutzeri), 5 Pseudomonas fluorescens (P. fluorescens), 4 Pseudomonas putida (P. putida), and 3 Pseudomonas aeruginosa (P. aeruginosa) isolates. Microflex LT identified all Pseudomonas isolates (100%) correctly with a score value ≥ 2.00. PCA positively discriminated the identified isolates into various groups. The antimicrobial resistance levels against Pseudomonas isolates were 81.16% for nitrofurantoin, 71% for ampicillin and ampicillin/sulbactam, 65.22% for cefuroxime and ceftriaxone, 55% for aztreonam, and 49.28% for ciprofloxacin. The susceptibilities were 100% for cefotaxime, 98.55% for ceftazidime, 94.20% for each piperacillin/tazobactam and cefepime, 91.3% for cefazolin. In conclusion, chicken meat was found to be contaminated with different Pseudomonas spp., with high incidence rates of P. lundensis. Microflex LT is a potent tool for distinguishing Pseudomonads at the species level.


Introduction
The nutrients in meat, including proteins, essential fatty acids, vitamins, and minerals, make it one of the most important food sources. As well as being highly active in water, it is highly susceptible to spoilage by microorganisms (Wickramasinghe et al. 2019). During and after the slaughtering process, meat can become contaminated with microbes (Bantawa et al. 2018). As strict procedures exist to ensure quality in the meat industry, the transportation and storage of meat has become a major source of contamination with microbes that harm human health (Kennedy et al. 2005;Nychas et al. 2008;Rouger et al. 2017). Meat and its products carry various microbiological dangers, which significantly increase the risk of infection and death, especially in developing countries (Lianou et al. 2017).

Open Access
*Correspondence: aymanella2007@yahoo.com Elbehiry et al. AMB Express (2022) 12:53 Spoilage bacteria are commonly found in raw meat before the slaughter process, and they can invade the meat during the handling, carriage, or packing process. (Doulgeraki et al. 2012). Food processing can be a main source of the food chain contamination, particularly for fresh foods or products that are not subjected to heat treatments or other sanitization during its preparation. Pseudomonas is an adaptable microorganism in the food processing environment (Stellato et al. 2017). As a source of meat contamination with Pseudomonas, poor sanitation of meat shops and unhygienic processing and unawareness of meat retailers of basic requirements and guidelines of meat shop, can be identified (Bantawa et al. 2018).
Among the important microbes that lead to the contamination of meat and meat products are Pseudomonas, Brochothrix, Acinetobacter, and Shewanella, which have been recovered from frozen meat (Wickramasinghe et al. 2019). Of the genus Pseudomonas, P. fluorescens, P. fragi, P. lundensis, P. migulae, and P. putida are considered frequent species found in chilled meat (Doulgeraki et al. 2012). In general, most of Pseudomonas species can grow at temperatures below 7 °C (psychrotrophic) and are characterized by their capabilities to contaminate fresh food and the surrounding environment, especially in the absence of the necessary sterilization procedures (Stellato et al. 2017;Quintieri et al. 2019). Pseudomonas lundensis (P. lundensis) represents one of the most significant psychrotrophic microorganisms that leads to deterioration in frozen meat (Liu et al. 2015). P. lundensis is a gram-negative psychrotrophic motile bacterium that can grow at temperatures fluctuating from 0 to 33 °C (Ercolini et al. 2010). In addition, previous studies carried out by Caldera et al. (2016) and Raposo et al. (2017) demonstrated that most Pseudomonas species have the capacity to release different thermotolerant proteolytic and lipolytic enzymes that can seriously decrease the quality and shelf life of meat and its products.
Although its ability to produce fluorescent pigments, P. lundensis may appear to be confusing when compared to non-pigment species (such as P. fragi). Further studies have revealed P. lundensis to be strictly associated with both the P. fragi and the P. fluorescens groups. During the stowage process, these bacteria form unpleasant odours and slime, causing meat to deteriorate (Wickramasinghe et al. 2019). Nevertheless, P. lundensis has predominantly been associated with milk and meat putrefaction, and new studies have utilized culture techniques and established that it exists in patients' lungs, particularly in patients suffering from cystic fibrosis (Scales et al. 2018). Nonetheless, the role of P. lundensis in lung deterioration and its probable role in respiratory distress are still unidentified. It is worth noting that in contrast to other microbes that cannot grow at low temperatures, psychrotrophic Pseudomonads have the ability to adapt and rapidly colonize ice-cold foods, leading to deterioration and biofilm formation (De Jonghe et al. 2011;Quintieri et al. 2019;Orellana-Saez et al. 2019). This later action increases their adaptability and scattering capacity, and as a result, measures to eliminate them can provoke and increase their resistance to various antimicrobial drugs. As a consequence of these features, the existence of Pseudomonas spp. such as P. lundensis, P. fragi, P. fluorescens, P. gessardii, and P. taetrolens in hilled fresh food products has been developing great attention (Baruzzi et al. 2012;Guidone et al. 2016;Brasca et al. 2018;Quintieri et al. 2019).
Nevertheless, culture-independent techniques supply a broader viewpoint on bacterial assortment, and culturing novel isolates remains significant and habitually accomplished in the majority of microbiological laboratories. This is predominantly correct for ecological bacteria, which are considered a huge source of new natural products for feed flavours, and in the field of developing medicines and other manufacturing products (Stafsnes et al. 2013;Timperio et al. 2017). To recognize and categorize new isolates at the genus and species levels, numerous techniques, such as phenotypic and genotypic methods, exist for this purpose. However, while these methods are considered the gold standard for the identification of different types of microorganisms, they cannot provide adequate and reliable data regarding the detection and discrepancy of various bacteria at the species level (Pesciaroli et al. 2015).
Therefore, it is necessary to use a fast and accurate technique such as mass spectrometry technology to recognize and distinguish different microbes isolated from food products. MALDI-TOF MS is an extraordinary throughput-dependent tool utilized for protein analysis. Previous studies have proven that the analysis of complete bacterial cells using the technique of protein analysis is one of the most important methods employed in identifying different microbes in the past ten years. . However, the challenge in the application of this technology in bacterial identification and grouping is the accessibility of cost-effective devices delivered with powerful datasets and easy software (Emonet et al. 2010;Elbehiry et al. 2017).
Nevertheless, the initial utilization of MALDI-TOF MS for the detection of several microorganisms, including bacteria and fungi, was not commonly used 30 years ago due to the absence of satisfactory databases (Tshikhudo et al. 2013). Recently, MALDI-TOF MS has been able to classify and discriminate psychrotrophic bacteria at both the genus and species levels by matching the spectral profiles of field isolates with stored spectral proteins from reference strains (Vithanage et al. 2014;Dong 2020). The workflow of MALDI-TOF MS is based mainly on dissolving a fresh bacterial colony in an appropriate matrix compound and then inoculating it onto a target plate for protein analysis using laser shots in a measuring chamber. As a final point, a mass spectrum is obtained and displayed using particular software .
Recently, antimicrobial resistance of different microorganisms has become an urgent matter due to their direct impact on public health worldwide. It is known that antibiotic-resistant bacteria have a close relationship with infections in hospitals, and P. aeruginosa is one of the most important opportunistic bacteria that affect human health, particularly in patients with defective immune systems (Chatterjee et al. 2016;Quintieri et al. 2019).
Furthermore, current suggestions emphasize that nonvirulent Pseudomonads not only have the ability to cause infections in the bloodstream of humans but also exhibit numerous types of multidrug resistance against various classes of antibiotics, which is a source of great danger to human health as a result of their high adaptability (Chatterjee et al. 2016;Cole and Singh 2017). Numerous Pseudomonas spp. of food origin are competent to resist various antimicrobial agents of various classes, especially β-lactams such as penicillins, cephalosporins, carbapenems, and monobactams (King et al. 2014). The objective of the present investigation was to identify Pseudomonas spp. recovered from chicken meat samples using a Microflex LT device and to examine the antimicrobial resistance of Pseudomonas against various antimicrobial agents using AST GN83 cards.

Sample collection
A total of 320 frozen chicken meat products (200 g of each sample) represented by breast, thigh, burger, and nuggets (80 of each) were randomly collected from various retail stores in the Al-Qassim region, Saudi Arabia, at various intervals from June to December 2020. Each sample was preserved independently in a Ziploc ® brand freezer bag at 4 ºC, and all samples were then transferred directly to the microbiology laboratory in a heat-insulated ice box under the appropriate hygienic conditions for bacteriological examination.

Sample processing and isolation of Pseudomonas spp.
According to the guidelines provided by the Feng et al. (2002), 25 g of each sample was moved into a sterilized container with 225 ml of sterile peptone water (0.1%) under strict hygienic measures, and homogenization was performed using a Denville Ultra EZgrind ™ Tissue Homogenizer (Thomas Scientific, USA) at 14,000 rpm for 3 successive minutes and was then incubated for 5 min at 25 °C. From this mixture, 1 ml was moved into a sterilized test tube containing 9 ml of sterile peptone water, from which tenfold (1:10) serial dilutions were processed. The prepared samples were subjected to isolation and determination of Pseudomonas counts (ISO 2003). In brief, 0.1 ml of each homogenized sample was independently inoculated into duplicate Petri dishes on Thermo Scientific ™ Remel ™ Pseudomonas Isolation Agar supplemented with glycerol and uniformly distributed with a sterile plastic spreader (Thomas Scientific, USA). The inoculated plates were incubated at 4 °C and 25 °C for a couple of days. Then, greenish yellow colonies were detected and enumerated. The average count was considered and recorded from serial dilutions of 10 -3 to 10 -6 . Subculturing of all suspected colonies was carried out by streaking on nutrient agar and incubating at 4 °C for 3 to 5 days to obtain purified colonies. All purified strains were kept in the CRYOBANK ™ Bacterial Culture Freezing System (COPAN Diagnostics Inc., Murrieta, USA) for further investigations.

Phenotypic identification of Pseudomonas species Microscopy and Gram stain properties
All purified strains kept in Cryobank vials were subcultured again for microscopic identification of Pseudomonas species using the Gram staining technique (Becerra et al. 2016).
In brief, a fresh colony of each strain was fixed onto a clean, dried slide, and then the colony was flooded with different chemicals. Crystal violet dye was first dropped onto the glass slide containing bacterial cells, and then iodine was added to fix the dye. Ethanol was then added to remove the dye from unspotted cells, and safranin was added as a final point to stain the gram-negative bacteria. The stained slides were scanned by light microscopy using an oil immersion lens to observe the morphology of bacteria. The isolates were recognized as gram-negative if they appeared pink.

Enzymatic activities
The enzymatic activities of Pseudomonas species were evaluated using certain biochemical tests, including oxidase, citrate utilization and indole tests (LaBauve and Wargo 2012). The oxidase test was performed by smearing a fresh colony of each isolate onto a sterile oxidase filter paper disc (Sigma-Aldrich, USA) soaked in distilled water. The positive oxidase activity results are indicated by the appearance of a purple colour. The capacity of Pseudomonas spp. to utilize citrate as a source of energy was carried out by streaking a fresh purified colony onto a Simmons citrate agar (Sigma-Aldrich, USA) slant and incubated at 37 °C for 5-7 successive days. Citrate utilization was indicated by the appearance of a sky-blue colour.
The capability of Pseudomonas spp. to convert tryptophan into indole was tested by inoculation of the suspected organism into tryptophan broth (Sigma-Aldrich Chemie GmbH, Germany), which was then incubated at 37 °C for a couple of days. Thereafter, using gentile agitation, 0.5 ml of Kovacs reagent was added until a redviolet colour appeared, indicating positive results, while a yellow colour indicates negative results.

Identification and determination of antimicrobial resistance via the Vitek 2 Compact system
All gram-negative isolates that showed positive results for both citrate utilization and oxidase tests and negative indole tests were further examined by the Vitek 2 Compact system (bioMerieux, France) for confirmation of species identification and antimicrobial resistance. Briefly, preparation of the isolate suspension was carried out and then adjusted using McFarland standards (0.5 to 0.63) as stated in the company's instructions. AST-GN83 gram-negative identification cards, which included 18 antimicrobial drugs, were utilized as gramnegative antibiotic susceptibility cards for Pseudomonas spp. (Table 1). According to the company's instructions, Vitek ® 2 cards were inoculated, and then the isolate IDs were submitted to the device to permit the selection of precise interpretive standards. Based on the authorizations of the Clinical and Laboratory Standards Institute (CLSI) ( According to the method previously described by Barreiro et al. (2010), Microflex LT (Bruker Daltonics, Bremen, Germany) was applied for the recognition and classification of Pseudomonas species from chicken meat samples. All isolates were analysed using both FlexControl and Compass software (Flex Series version 1.3). All isolates were prepared by culturing on nutrient agar (Sigma-Aldrich, USA) followed by incubation for a couple of days at 37 °C. The ethanol/formic acid extraction procedure was utilized as stated by Bruker Daltonics. Briefly, 2 pure colonies were relocated onto a clean Eppendorf tube holding 300 µl of sanitized water and 900 µl of ethanol (99.9%). The contents were mixed carefully by centrifugation at 13,000 rpm for 2 mins. The obtained pellet was dried in air for 5 min after the removal of the supernatant. Fifty microlitres of formic acid (70%) was added to the air-dried pellet, and acetonitrile (70%) was then added after proper mixing for 2 min at 13,000 rpm. One microlitre of the supernatant for each isolate was then placed onto a target plate of Microflex LT and left to dry at 25 °C. Subsequently, 1 µl of matrix solution αcyano-4 hydroxy-cinnamic acid was added. The target plate was then submitted to the Microflex LT machine for identification and data reading. A bacterial test standard (Escherichia coli) was used as a positive control throughout the experiment.
The score values of indeterminate spectra were compared with the reference spectra stored in the databank. Microflex LT has the capacity to accurately recognize and distinguish different microorganisms when the values range from 2 to 3. However, misidentification can result if this value ≤ 1.69. The diverse spectra created by IVD Compass Software were analysed via a m/z range from 2000 Da to 20,000 Da. A dendrogram could be produced from the main spectral profile (MSP) database, which includes > 6.989 different species of bacteria and fungi.

Proteomic analysis of Pseudomonas spp.
In the existing study, the isolated strains were screened by Microflex LT, and the spectra of the field isolates were parallel to the reference spectra. According to the results obtained, Microflex LT was capable of verifying all Pseudomonas spp. by 100%. Analysing these results shows that approximately 20 prominent ion peaks were detected in the original bands from the region varying from 2000 to 10,200 Daltons (Da) (Fig. 1A), which were confirmed from the gel view (Fig. 1B), and robust peaks were revealed at 3800, 3860, 4440, and 4550 Da ( Fig. 2A), which were confirmed from the gel view (Fig. 2B). All 69 strains of Pseudomonas spp. were correctly identified as follows: 18 P. lundensis, 16 P. fragi, 13 P. oryzihabitans, 10 P. stutzeri, 5 P. fluorescens, 4 P. putida, and 3 P. aeruginosa. All of these species were synchronized with the P. Lundensis DSM 6252 T HAM (Fig. 3), P. fragi DSM 3456 T HAM, P. oryzihabitans DSM 6835 T, P. stutzeri V319 MCRF, P. fluorescens DSM 1976, P. putida ATCC 49,128 THL, and P. aeruginosa DSM 1117 reference strains stored in Compass IVD software. All Pseudomonas strains were distinguished by matching their spectra with the Bruker database, which includes 70 strains obtained from the American Type Culture Collection (ATCC) and the German Collection of Microorganisms and Cell Cultures GmbH (DSMZ).

Discussion
The contamination of chilled meat with various microbes is one of the major causes of cost-effective problems in meat production and has an impact on public health worldwide (Wickramasinghe et al. 2019). Despite the  use of modern methods of meat preservation, microbial contamination remains a major threat. Psychrotrophic Pseudomonas spp. are considered the main bacteria that lead to putrefaction of ice-cold meat under aerobic conditions. The genus Pseudomonas is one of the most polluting microbes and is characterized by its great ability to withstand difficult environmental conditions, which leads to the prevention of the growth of other microorganisms. To diminish contamination of meat, proper detection and treatment of various Pseudomonas spp. are critical. Therefore, this study concentrated on an accurate method of identification and differentiation of Pseudomonas spp. and evaluated their degrees of resistance and susceptibility to various antibiotics commonly used for treatment.
Based on our results, the mean Pseudomonas counts (CFU/g) were 10.1 × 10 3 ± 1.45 × 10 3 , 7.4 × 10 3 ± 0.89 × 10 3 , 6.5 × 10 3 ± 6.43 × 10 3 and 4.3 × 10 3 ± 7.56 × 10 3 for the isolates recovered from the breast, thigh, burger, and nuggets, respectively. Similar findings were recorded by Hassan et al. (2020), who found that the mean Pseudomonas counts recovered from various chicken meat products (chilled breast, thigh, nuggets, and burger) varied from 3.51 × 10 3 ± 0.76 × 10 3 to 8.44 × 10 3 ± 1.85 × 10 3 . Other parallel records detected by Morshdy et al. (2018) and Abd El-Aziz (2015) were 3.6 × 10 3 and 2.6 × 10 4 , respectively. Although, the findings of the current study are similar to those of previous studies, the practice of comparing CFU/g of bacteria in meat samples across multiple studies is unusual because CFU is highly dependent on storage conditions, sampling preparation, and slaughter methods. Although the research performed by Hinton et al. (2007) indicated that psychrotrophic bacteria were not recovered from carcasses washed with chlorinated water, different species of Pseudomonas were the most predominant psychrotrophs recovered from all carcasses when stored in refrigerators for two weeks. Several investigations have revealed that the initial Pseudomonas count is directly associated with the period of storing meat in the refrigerator, and meat spoilage occurs when the number of Pseudomonas ranges from 10 7 to 10 8 (Hassan et al. 2020).
In addition, 11 strains of Pseudomonas species recovered from cooked chicken burgers were identified by Franzetti and Scarpellini (2007) as 8 strains of P. fragi, followed by 2 P. chicorii and 1 P. fluorescens. In contrast, P. aeruginosa was not detected in 100 chicken meat specimens (Iroha et al. 2011). In another study conducted by Caldera et al. (2016), the deterioration of food was commonly associated with P. aeruginosa, P. fragi, P. lundensis and P. fluorescens (Caldera et al. 2016). Moreover, Bellés et al. (2017) and Wang et al. (2017) clarified that the capability of these microorganisms to live at low temperatures may lead to trouble throughout the storage of foodstuffs. The existence of Pseudomonas spp. in various food samples is of high importance because this type of bacteria has a bad impact on human health and is considered a sign of food quality (Yagoub 2009).
Because phenotypic-based detection of various foodborne pathogens is difficult and takes a long time to be carried out, Microflex LT was meaningfully applied in our study for the initial detection and classification of numerous bacteria from chicken meat samples, as it is an easy, quick, specific, and inexpensive detection technique compared to other approaches (Singhal et al. 2015;van Belkum et al. 2017;Elbehiry et al. 2019). In recent times, Microflex LT has been discovered to be an imperative tool for the powerful recognition of microbial intimidations that may pollute both water and foodstuffs (Singhal et al. 2015;Elbehiry et al. 2019).
In the present investigation, the percentage of mass spectral identification of Pseudomonas strains was 100% for all 7 species of Pseudomonas. The interpreted results confirmed that all spectral profiles produced by Microflex LT IVD Compass Software were suitable to distinguish between Pseudomonads at the species level. The accurate identification observed in our study may be a result of the restructured database . Comparable findings were noted by Böhme et al. (2011), who applied Microflex LT effectively in the exact identification of gram-negative bacteria (e.g., Pseudomonas and Enterobacter) of different species recovered from seafood. Consequently, Microflex LT has been demonstrated to be an authoritative instrument for microbial identification. Höll et al. (2016) also identified several microorganisms isolated from packaged poultry meat using Microflex LT, and they found that Pseudomonas spp. is one of the most common bacteria found after 7 days of storage at 4 °C and 10 °C.
In addition, principal component analysis (PCA) generated by the Microflex LT device magnificently divided P. lundensis, P. fragi, P. oryzihabitans, P. stutzeri, P. fluorescens, P. putida, and P. aeruginosa strains into different groups. Han (2010) and Elbehiry et al. (2019) indicated that PCA is usually applied as a mathematical tool to extract and demonstrate the modification in the spectral profiles within the database.
The spread of antimicrobial resistance amongst the genus Pseudomonas was also examined in the current study. Of late, antimicrobial resistance represents one of the common public health problems, as multidrugresistant bacteria related to animals may be virulent and transferred simply to human beings through food chains and comprehensively dispersed through animal wastes to the environment (Manyi-Loh et al. 2018). Antimicrobial resistance is problematic and multifaceted and occurs as a consequence of the unreasonable use of antibiotics under poor hygienic measures (Osman et al. 2019).
In the present investigation, the AST GN83 card was applied to display the resistance and susceptibility of 69 Pseudomonas species recovered from various chicken meat samples against several antibiotics frequently utilized for the treatment of gram-negative pathogens. Based on our results, the majority of Pseudomonas isolates exhibited higher degrees of susceptibility to cefotaxime (100%), ceftazidime (98.55%), cefepime (94.2%), gentamycin (86.96%), and amikacin (82.16%). These findings were similar to those obtained by CLSI (2015). It was also observed that the majority of the Pseudomonas isolates were highly sensitive to meropenem (70%). Parallel results were achieved in previous studies carried out in Turkey by Shenoy et al. (2002) and Deniz Yilmaz et al. (2016) and in Kenya by Mwinyikombo (2018), who revealed that Pseudomonas isolates demonstrated higher degrees of susceptibility to both meropenem and imipenem. Nonetheless, other studies performed in India by Sivanmaliappan and Sevanan (2011) illustrated a higher degree of resistance to imipenem (66.6%), a finding that could be explained by the misuse of broad-spectrum antibiotics such as carbapenems.
There are many mechanisms through which pseudomonads gain multidrug resistance, including reduced outer membrane permeability (De Oliveira et al. 2013;Lavilla Lerma et al. 2014), beta-lactamase production, and multidrug efflux pumps with a broad substrate spectrum (Henwood et al. 2001;Lavilla Lerma et al. 2014). It has been suggested that the use of antimicrobials that can enhance gene transfer by enhancing the SOS system (Lima et al. 2020), as well as the presence of pathogens as potential reservoirs of resistance factors, may all contribute to an increase in antibiotic resistance in pseudomonas. Pathogenic bacteria like pseudomonas can grow in a wide variety of habitats, each of which has important variables that contribute to the evolution of their resistance (Pachori et al. 2019). Because many resistance genes are carried on plasmids or integrons, the spreading of multiple drugresistant pseudomonads from various sources to both people and the environment strongly suggests horizontal gene transfer as the primary pathway for dissemination of resistance determinants (Von Wintersdorff et al. 2016).
Based on the results of our study, we demonstrate the high incidence rate of P. lundensis, P. fragi, and P. oryzihabitans among different Pseudomonas species found in chicken meat samples. Microflex LT for the detection of Pseudomonas species proved to be a reliable, affordable, and easy-to-apply method during this investigation and PCA generated by Microflex LT enabled discrimination between different species of Pseudomonas. In future studies, it will be necessary to determine if this technique can be useful in recognizing and correcting discrepancies in Pseudomonas spp. in food samples. We also found that the various species of Pseudomonas are multidrug resistant. In this way, it is conceivable that resistance will evolve over time, which is why the number of antimicrobials is decreasing. Due to the potential threat posed by Pseudomonas, the transmission of resistance may negatively affect individuals.