Bacterial Histidine Kinase and the Development of Its Inhibitors in the 21st Century

Bacterial histidine kinase (BHK) is a constituent of the two-component signaling (TCS) pathway, which is responsible for the regulation of a number of processes connected to bacterial pathogenicity, virulence, biofilm development, antibiotic resistance, and bacterial persistence. As BHK regulation is diverse, inhibitors can be developed, such as antibiotic synergists, bacteriostatic/bactericidal agents, virulence inhibitors, and biofilm inhibitors. Inhibition of essential BHK has always been an amenable strategy due to the conserved binding sites of the domains across bacterial species and growth dependence. Hence, an inhibitor of BHK might block multiple TCS regulatory networks. This review describes the TCS system and the role of BHK in bacterial virulence and discusses the available inhibitors of BHK, which is a specific response regulator with essential structural features.


Introduction
Bacterial infections have a substantial effect on global health.However, the discovery of wonder medications known as "antibiotics" offered consistent health advantages, reduced infections and decreased patient mortality during the last decade [1].Moreover, the extensive use and misuse of antibiotics exacerbates selective pressure on microbes, leading to antimicrobial resistance (AMR).The global scope of the problem, as well as the impact of AMR on human health, health-care expenses, and society, remains largely unclear [2].AMR is a complicated worldwide public health concern, and no single or simple solution will suffice to fully control the emergence and spread of pathogenic organisms resistant to existing antibacterial medications [3].AMR is caused by a number of different mechanisms, such as drug or target inactivation (penicillinases, cephalosporinases, carbapenemases, and β-lactamases), binding site modifications (PBP2a in Staphylococcus aureus, which changes the cross-linking target of the peptidoglycan layer in Enterococcus faecium and Enterococcus faecalis), and the development of resistance to AMR (the reduced level of OprD porin protein in Pseudomonas aeruginosa exhibits resistance against imipenem) [4][5][6][7].In 2010, Neisseria, Staphylococcus, and Enterobacteriaceae developed resistance to the antibiotic ceftaroline (2010); Staphylococcus developed resistance to both linezolid (2000) and daptomycin (2003) in 2001; and Acinetobacter and Pseudomonas developed resistance to these antibiotics in 2004 and 2005, respectively.According to statistics from the WHO, 1.27 million patients died due to infections caused by resistant bacteria in 2019 [8][9][10].Furthermore, the mortality rate might increase to 10 million patients each year by 2050, as reported by O'Neill.Therefore, immediate action is needed to counteract the emergence and rampant dissemination of AMR [11].
Many targets have been investigated for the development of antibacterial drugs [1].The cell wall biosynthesis process has been widely investigated and validated as an antibacterial target of the β-lactam and glycopeptide classes of antibiotics [12].The fatty acid production pathway has also been validated by the widespread use of well-known medications such as isoniazid, an antitubercular treatment, and triclosan, an antiseptic [13].Bacterial folate biosynthesis is a well-known and appealing target that involves many types of enzymes.However, the well-known targets are DHFR (dihydrofolate reductase) and DHPS (dihydropteroate synthase).DHFR has been verified by the use of drugs such as trimethoprim (an antifolate antibiotic) and pyrimethamine (an antiprotozoal agent).DHPS is another target that has been proven to be crucial for folate synthesis and was validated as a sulfonamide [14].
Another potent antibacterial target is the dual inactivation of DNA GyrB and ParE.By inhibiting these topoisomerases, DNA replication, repair, and catenation are prevented [15].Furthermore, protein synthesis, primarily carried out by the molecular machinery known as ribosomes and translational machinery, is regarded as a vulnerable target for antibiotics [16].Tetracyclines are widely used antibacterial medications that target protein synthesis (blocking the A site of the 30S subunit of the ribosome, thereby preventing the binding of aminoacyl t-RNA) [17].Aminoglycosides interfere with the formation of initiation complexes of the 30S subunit [18].During the transpeptidation cycle, macrolides interfere with the elongation of peptides [19].Despite the fact that these antibiotics and their targets have been shown to be clinically significant, the increase in resistance necessitates the development of novel strategies.Several strategies already reported in the literature include structural modification, bacteriophage therapy, and targeting of the explored pathways with novel molecules.
None of these strategies were found to be effective in preventing AMR.Therefore, research is more focused on the discovery of novel untapped or unexplored pathways.One such attractive target is bacterial histidine kinases (BHKs).BHKs are constituents of bacterial two-component systems (TCSs), which are involved in primary signal transduction pathways.BHK is highly conserved among all bacterial species and has broad-spectrum activity.In addition, no human homologs or proteins with similar structures (with the exception that mammalian kinases possess comparable protein folds in the ATP domain) exhibit selectivity toward bacterial species [20].Furthermore, BHK is important for bacterial survival, the inhibition or inactivation of which results in bacterial death.All these characteristics make BHK a potential antibacterial target.In this review, we discussed the biological significance of TCS-BHKs in the identification of new antibacterial agents as well as existing TCS-BHK inhibitors, which can be used further to develop new and diverse antibacterial agents.

TCS Signaling Pathway and BHK
TCSs are considered appealing antibacterial targets because they are conserved in almost all bacterial species.In addition, the TCS is and involved in the regulation of a number of processes connected to bacterial pathogenicity, virulence, biofilm development, antibiotic resistance, and bacterial persistence.Although crucial for bacterial adaptability and fitness, only a few of these TCSs are considered essential for bacterial cell survival.However, some TCSs are not essential for bacterial survival in laboratory environments, but they enhance bacterial fitness by enabling adaptation to environmental changes.Certain responses are expressed by pathogenic bacteria in response to their host environment, and these responses typically rely on the TCS system.Another important consideration is the difference between targeting essential and nonessential TCSs in pathogens.Essential TCSs are essential for the survival and growth of bacteria.While inhibiting TCSs can efficiently kill or suppress bacteria, it can also lead to the swift development of resistance, as bacteria are under strong selective pressure to survive.On the other hand, nonessential TCSs often regulate virulence factors rather than basic survival.By targeting these systems, we can reduce the pathogen's ability to cause disease without necessarily killing it, which may result in slower resistance development.For example, studies have shown that targeting the Agr system in Staphylococcus aureus, which is not essential for survival but crucial for virulence, can significantly diminish its ability to cause infections without inducing rapid resistance [21,22].This approach could offer a more sustainable way to manage bacterial infections.TCS signaling involves autophosphorylation of a membrane-bound BHK, phosphotransfer of the phosphoryl group to a cognate response regulator (RR), and ultimately modulation of the expression of target genes (Figure 1) [23].BHKs are present in both essential and nonessential TCSs.Appropriate phosphorylation levels of RR are tightly regulated by the phosphatase activity of BHK, RR, or a partner protein [23,24].BHK autophosphorylation is mediated via the catalytic and ATP-binding (CA) domain, which binds ATP and phosphorylates BHK at a conserved histidine residue in the dimerization and histidine phosphotransfer (DHp) domain.The CA and DHp domains are conserved and present in all HKs, whereas the remaining sensor domains (periplasmic, PAS, GAF, HAMP) are variable and not present in all HKs [23].
survival.However, some TCSs are not essential for bacterial survival in laboratory environments, but they enhance bacterial fitness by enabling adaptation to environmental changes.Certain responses are expressed by pathogenic bacteria in response to their host environment, and these responses typically rely on the TCS system.Another important consideration is the difference between targeting essential and nonessential TCSs in pathogens.Essential TCSs are essential for the survival and growth of bacteria.While inhibiting TCSs can efficiently kill or suppress bacteria, it can also lead to the swift development of resistance, as bacteria are under strong selective pressure to survive.On the other hand, nonessential TCSs often regulate virulence factors rather than basic survival.By targeting these systems, we can reduce the pathogen's ability to cause disease without necessarily killing it, which may result in slower resistance development.For example, studies have shown that targeting the Agr system in Staphylococcus aureus, which is not essential for survival but crucial for virulence, can significantly diminish its ability to cause infections without inducing rapid resistance [21,22].This approach could offer a more sustainable way to manage bacterial infections.TCS signaling involves autophosphorylation of a membrane-bound BHK, phosphotransfer of the phosphoryl group to a cognate response regulator (RR), and ultimately modulation of the expression of target genes (Figure 1) [23].BHKs are present in both essential and nonessential TCSs.Appropriate phosphorylation levels of RR are tightly regulated by the phosphatase activity of BHK, RR, or a partner protein [23,24].BHK autophosphorylation is mediated via the catalytic and ATP-binding (CA) domain, which binds ATP and phosphorylates BHK at a conserved histidine residue in the dimerization and histidine phosphotransfer (DHp) domain.The CA and DHp domains are conserved and present in all HKs, whereas the remaining sensor domains (periplasmic, PAS, GAF, HAMP) are variable and not present in all HKs [23].The BHK CA domain is a desirable target for structure-based virtual screening and phenotypic screening of pharmacological inhibitors due to its conserved properties and crucial function in TCS signal transduction.The high level of sequence conservation in the CA catalytic site further suggests that inhibitors directed against this region will have broad-spectrum antibacterial effects.The CA domain is thus a promising BHK target location for the discovery and development of broad-spectrum antibiotics.Drug polypharmacology, which involves simultaneous inhibition of many targets, has been suggested The BHK CA domain is a desirable target for structure-based virtual screening and phenotypic screening of pharmacological inhibitors due to its conserved properties and crucial function in TCS signal transduction.The high level of sequence conservation in the CA catalytic site further suggests that inhibitors directed against this region will have broadspectrum antibacterial effects.The CA domain is thus a promising BHK target location for the discovery and development of broad-spectrum antibiotics.Drug polypharmacology, which involves simultaneous inhibition of many targets, has been suggested as a method to prevent the emergence of drug resistance to novel antibiotics [25][26][27][28].Because bacteria have several TCSs, inhibitors of the highly conserved CA domain are likely to shut down a number of signaling pathways, impairing the bacteria's capacity to quickly adapt to environmental changes, including those that occur during an infection of the host.TCS inhibition may not be bactericidal for some bacteria, but it is likely to limit efficient growth, lowering survival capacity [23] (Figure 1).The ATP-binding Bergerat fold found in the CA domain of many human protein families, which is also present in essential proteins such as Hsp90, is one potential drawback of BHKs.The Bergerat fold may cause BHK autophosphorylation inhibitors (HKAIs) to have off-target effects on human ATP-binding domains and may also cause toxicity to mammalian cells.This fold is present in both microbial and human ATP-binding protein domains [29].

TCS-BHK Inhibitors
For almost 20 years, TCSs have been identified as viable antibacterial therapeutic targets.Some TCSs are essential or required for bacterial growth.Furthermore, given the high degree of conservation among TCS active sites and the occurrence of several TCSs in every bacterium, an inhibitor with broad-spectrum activity that targets various TCS regulatory networks should be identified.Overall, targeting TCSs is likely to effectively disable bacteria's ability to adapt to environmental and physiological changes.The availability of crystal structures of BHK has made the design of BHK inhibitors possible.In the current review, we discussed novel BHK inhibitors with different response regulators identified in the literature (Table 1).In 2022, Radwan et al. synthesized a series of novel isatin derivatives with either β-hydroxyketone or chalcone moieties and examined their antibacterial activity.These compounds (1a-1j) (Figure 2) exhibited potent activity against S. aureus in the range of 0.044-0.057mmol/L (MIC).Among these compounds, 1a showed the most potent antibacterial activity, with an MIC of 0.026 mmol/L.The activity of 1a against S. aureus was explained by its significant docking score values (glide score −36.231 kcal mol −1 , electrostatic energy −0.697 kcal mol −1 , and van der Waals energy −35.534 kcal mol −1 ) within the binding site of BHK (S. aureus) (PDB: 5C93).Compound 1a could be further optimized for the development and synthesis of more potent antibacterial agents [48].
Focusing on the discovery of novel antibacterial agents in 2020, Carabajal et al. screened 686 compounds from the published kinase inhibitor set (PKIS), a compound library published by GlaxoSmithKline, to identify inhibitors of PhoP/PhoQ in S. typhimurium.The results demonstrated that a series of compounds with quinazoline scaffolds exhibited potent and selective downregulation of PhoP/PhoQ-activated genes.Among these quinazoline derivatives, 2a and 2b (Figure 3) showed more potent antibacterial activity, with IC 50 values of 6.9 and 3.2 µM, respectively.Furthermore, these compounds can emerge as appealing lead molecules for the development of antibacterial agents [49].
In an effort to discover novel antibacterial agents, waldiomycin (3a) and its methyl ester derivative (3b) (Figure 4) were identified as novel BHK inhibitors.Waldiomycin, a methyl ester derivative, exhibited significant inhibitory activity against the Walk-type H-box region, with IC 50 values of 10.2 and 75.8 µM, respectively.The results demonstrated that the binding interactions of ligands with WalK-BHK could be studied further for the development of novel antibacterial agents [50].
In another study by Mizar et al. in 2018, xanthoangenol B 1 (4a) was identified using a GFP (green fluorescent protein) reporter system that was previously used to identify SaeRS TCS (response regulator in S. aureus) inhibitors obtained from plants.Approximately four derivatives (xanthoangenol (4b), xanthoangenol (4c) and PM-56 (4d)) (Figure 5) were identified and screened for their antibacterial activity.Among them, 4a and 4d demonstrated excellent inhibitory activity against SaeRS, with IC 50 values of 2.1 and 4.3 µM, respectively [51].
activity, with an MIC of 0.026 mmol/L.The activity of 1a against S. aureus was ex by its significant docking score values (glide score −36.231 kcal mol −1 , electrostatic −0.697 kcal mol −1 , and van der Waals energy −35.534 kcal mol −1 ) within the bindin BHK (S. aureus) (PDB: 5C93).Compound 1a could be further optimized for the d ment and synthesis of more potent antibacterial agents [48].ibiotics 2024, 13, x FOR PEER REVIEW Focusing on the discovery of novel antibacterial agents in 20 screened 686 compounds from the published kinase inhibitor set (PK brary published by GlaxoSmithKline, to identify inhibitors of PhoP murium.The results demonstrated that a series of compounds with qu exhibited potent and selective downregulation of PhoP/PhoQ-activa these quinazoline derivatives, 2a and 2b (Figure 3) showed more pote tivity, with IC50 values of 6.9 and 3.2 µM, respectively.Furthermore, th emerge as appealing lead molecules for the development of antibacter In an effort to discover novel antibacterial agents, waldiomycin ester derivative (3b) (Figure 4) were identified as novel BHK inhibito methyl ester derivative, exhibited significant inhibitory activity agains box region, with IC50 values of 10.2 and 75.8 µM, respectively.The re that the binding interactions of ligands with WalK-BHK could be stu development of novel antibacterial agents [50].In 2019, Zhang et al. developed a system based on artificial proteoliposomes and used it for screening AgrC inhibitors.A library of traditional Chinese medicine (TCM) monomers was selected and screened for ArgC inhibitory activity.The results showed that the two TCM monomers rhein (5a) and aloe emodin (5b) (Figure 6) inhibited AgrC autophosphorylation with IC 50 values of 13.7 and 62.2 µM, respectively.Furthermore, these compounds inhibited the growth of S. aureus in a dose-dependent manner, with MIC values of 32 and 64 µg/mL, respectively [52].
In an effort to discover novel antibacterial agents, waldiomycin (3a) and its ester derivative (3b) (Figure 4) were identified as novel BHK inhibitors.Waldiom methyl ester derivative, exhibited significant inhibitory activity against the Walkbox region, with IC50 values of 10.2 and 75.8 µM, respectively.The results demon that the binding interactions of ligands with WalK-BHK could be studied further development of novel antibacterial agents [50].In 2019, Zhang et al. developed a system based on artificial proteoliposomes and used it for screening AgrC inhibitors.A library of traditional Chinese medicine (TCM) monomers was selected and screened for ArgC inhibitory activity.The results showed that the two TCM monomers rhein (5a) and aloe emodin (5b) (Figure 6) inhibited AgrC autophosphorylation with IC50 values of 13.7 and 62.2 µM, respectively.Furthermore, these compounds inhibited the growth of S. aureus in a dose-dependent manner, with MIC values of 32 and 64 µg/mL, respectively [52].In 2016, Velikova et al. reported the identification of putative BHK autophosphorylation inhibitors by combining in silico and in vitro fragment-based screening.Among the screened fragments, compound 6 (Figure 7) was the most potent compound, inhibiting  In 2019, Zhang et al. developed a system based on artificial proteoliposomes a it for screening AgrC inhibitors.A library of traditional Chinese medicine (TCM mers was selected and screened for ArgC inhibitory activity.The results showed two TCM monomers rhein (5a) and aloe emodin (5b) (Figure 6) inhibited AgrC au phorylation with IC50 values of 13.7 and 62.2 µM, respectively.Furthermore, the pounds inhibited the growth of S. aureus in a dose-dependent manner, with MIC of 32 and 64 µg/mL, respectively [52].In 2016, Velikova et al. reported the identification of putative BHK autophosphorylation inhibitors by combining in silico and in vitro fragment-based screening.Among the screened fragments, compound 6 (Figure 7) was the most potent compound, inhibiting the autophosphorylation of BHK in a concentration-dependent manner, with IC 50 s against S. aureus and E. coli BHK PhoR of 212 and 16 µM, respectively [31].
In 2016, Velikova et al. reported the identification of putative BHK autopho lation inhibitors by combining in silico and in vitro fragment-based screening.Am screened fragments, compound 6 (Figure 7) was the most potent compound, inh the autophosphorylation of BHK in a concentration-dependent manner, with IC50s S. aureus and E. coli BHK PhoR of 212 and 16 µM, respectively [31].Continued efforts to increase the potency of molecules against BHK led to the discovery of novel heterocycles.In 2017, Vo et al. demonstrated that repurposing diaryl pyrazolebased ATP-competitive (HSP90) inhibitors as effective antibacterial agents targeting BHKs is a promising strategy for the development of newer antibiotics.A total of nine CCT018159 (7a, Figure 8) derivatives were synthesized and evaluated against multiple BHKs (PhoQ, DivJ, and Cck).Compounds 7b, 7c, and 7d (Figure 8) showed favorable properties, both for the inhibition of CckA (C.crescentus) and PhoQ (Salmonella), which are essential for virulence.The results confirmed that the presence of a chlororesorcinol ring was essential for potent activity within the series.In summary, this study identified a pathway for the development of HSP90 inhibitors as novel antibacterial agents [30].targeting BHKs is a promising strategy for the development of newer antibiotics.A total of nine CCT018159 (7a, Figure 8) derivatives were synthesized and evaluated against multiple BHKs (PhoQ, DivJ, and Cck).Compounds 7b, 7c, and 7d (Figure 8) showed favorable properties, both for the inhibition of CckA (C.crescentus) and PhoQ (Salmonella), which are essential for virulence.The results confirmed that the presence of a chlororesorcinol ring was essential for potent activity within the series.In summary, this study identified a pathway for the development of HSP90 inhibitors as novel antibacterial agents [30].In 2017, Zheng et al. used whole-cell phenotypic high-throughput screening to screen a small-molecule library of approximately 540,000 compounds to identify new DosRST inhibitors.Compounds 8a and 8b (Figure 9) were identified as potential antibacterial agents.Compound 8a reduced the autophosphorylation of DosS with an IC50 of 1.9 µM, and 8b inhibited the autophosphorylation of both DosS and DosT with IC50s of 0.5 and 5 µM, respectively [53].In 2016, Boibessot et al. synthesized a series of thiophene derivatives and screened them for their antibacterial activity.Among them, eight compounds (9a-9h) (Figure 10) were found to inhibit the autophosphorylation activity of the BHKs WalK, PhoR, and ResE from B. subtilis, with IC50 values ranging from 52.81-196.9,1.63-122.6,and 20.3-243.9µM, respectively.These lead compounds can be used as a starting point for the development of novel antibacterial agents [36].targeting BHKs is a promising strategy for the development of newer antibiotics.A total of nine CCT018159 (7a, Figure 8) derivatives were synthesized and evaluated against multiple BHKs (PhoQ, DivJ, and Cck).Compounds 7b, 7c, and 7d (Figure 8) showed favorable properties, both for the inhibition of CckA (C.crescentus) and PhoQ (Salmonella), which are essential for virulence.The results confirmed that the presence of a chlororesorcinol ring was essential for potent activity within the series.In summary, this study identified a pathway for the development of HSP90 inhibitors as novel antibacterial agents [30].In 2017, Zheng et al. used whole-cell phenotypic high-throughput screening to screen a small-molecule library of approximately 540,000 compounds to identify new DosRST inhibitors.Compounds 8a and 8b (Figure 9) were identified as potential antibacterial agents.Compound 8a reduced the autophosphorylation of DosS with an IC50 of 1.9 µM, and 8b inhibited the autophosphorylation of both DosS and DosT with IC50s of 0.5 and 5 µM, respectively [53].In 2016, Boibessot et al. synthesized a series of thiophene derivatives and screened them for their antibacterial activity.Among them, eight compounds (9a-9h) (Figure 10) were found to inhibit the autophosphorylation activity of the BHKs WalK, PhoR, and ResE from B. subtilis, with IC50 values ranging from 52.81-196.9,1.63-122.6,and 20.3-243.9µM, respectively.These lead compounds can be used as a starting point for the development of novel antibacterial agents [36].In 2016, Boibessot et al. synthesized a series of thiophene derivatives and screened them for their antibacterial activity.Among them, eight compounds (9a-9h) (Figure 10) were found to inhibit the autophosphorylation activity of the BHKs WalK, PhoR, and ResE from B. subtilis, with IC 50 values ranging from 52.81-196.9,1.63-122.6,and 20.3-243.9µM, respectively.These lead compounds can be used as a starting point for the development of novel antibacterial agents [36].In 2015, Wilke et al. elucidated the active site of BHK using an HTS-FP displacement assay.The results demonstrated that nine compounds exhibited potential inhibitory activity against different BHKs.Among them, four compounds (11a-10d) (Figure 12) containing adenine moieties possess significant targetable inhibitor space within the binding pocket.The other five compounds (11e-10i) (Figure 12) that possess unique chemical  In 2015, Wilke et al. elucidated the active site of BHK using an HTS-FP displacement assay.The results demonstrated that nine compounds exhibited potential inhibitory activity against different BHKs.Among them, four compounds (11a-10d) (Figure 12) containing adenine moieties possess significant targetable inhibitor space within the binding pocket.The other five compounds (11e-10i) (Figure 12) that possess unique chemical In 2015, Wilke et al. elucidated the active site of BHK using an HTS-FP displacement assay.The results demonstrated that nine compounds exhibited potential inhibitory activity against different BHKs.Among them, four compounds (11a-11d) (Figure 12) containing adenine moieties possess significant targetable inhibitor space within the binding pocket.
The other five compounds (11e-11i) (Figure 12) that possess unique chemical structures were found to be more potent, as evidenced by their IC 50 values.These compounds could be utilized for the production of multitargeted, TCS-mediated antibiotics with innovative modes of action [46].
Antibiotics 2024, 13, x FOR PEER REVIEW 10 of 18 structures were found to be more potent, as evidenced by their IC50 values.These compounds could be utilized for the production of multitargeted, TCS-mediated antibiotics with innovative modes of action [46].13) that had potent inhibitory activity against PrrBA TCA, which is required for the viability of M. tuberculosis.Over 40 diarylthiazole derivatives, such as 12a and 12b, which demonstrated remarkable antibacterial activities with MICs of 0.4 and 0.25 µg/ml, respectively, were subsequently developed, and the majority of these derivatives exhibited favorable physicochemical characteristics and significant MICs against M. tuberculosis (MIC ≤1 µg/mL) [55].In 2014, Bellale et al. discovered a particular class of diarylthiazole compounds (Figure 13) that had potent inhibitory activity against PrrBA TCA, which is required for the viability of M. tuberculosis.Over 40 diarylthiazole derivatives, such as 12a and 12b, which demonstrated remarkable antibacterial activities with MICs of 0.4 and 0.25 µg/mL, respectively, were subsequently developed, and the majority of these derivatives exhibited favorable physicochemical characteristics and significant MICs against M. tuberculosis (MIC ≤1 µg/mL) [55].
Antibiotics 2024, 13, x FOR PEER REVIEW 10 of 18 structures were found to be more potent, as evidenced by their IC50 values.These compounds could be utilized for the production of multitargeted, TCS-mediated antibiotics with innovative modes of action [46].In 2014, Bellale et al. discovered a particular class of diarylthiazole compounds (Figure 13) that had potent inhibitory activity against PrrBA TCA, which is required for the viability of M. tuberculosis.Over 40 diarylthiazole derivatives, such as 12a and 12b, which demonstrated remarkable antibacterial activities with MICs of 0.4 and 0.25 µg/ml, respectively, were subsequently developed, and the majority of these derivatives exhibited favorable physicochemical characteristics and significant MICs against M. tuberculosis (MIC ≤1 µg/mL) [55].In 2012, Watanabe et al. screened more than 10,000 Streptomyces extracts by using differential growth assays and identified signermycin B (14) (Figure 15) as a potent compound that interfered with the WalK dimerization domain.Furthermore, its inhibitory activity against WalK was evaluated for different bacterial species (S. aureus, E. faecalis, B. subtilis, and S. mutans), and IC50 values ranging from 37-62 µM were calculated.These results demonstrated that the WalK dimerization domain could serve as a potent binding site, and further optimization of singermycin B could lead to the development of novel antibacterial agents [40].In another study, Cai et al. in 2011, identified four compounds, 15a-15d (Figure 16), as possible PhoQ inhibitors using HTS and enzymatic activity-coupled assays.These four In 2012, Watanabe et al. screened more than 10,000 Streptomyces extracts by using differential growth assays and identified signermycin B (14) (Figure 15) as a potent compound that interfered with the WalK dimerization domain.Furthermore, its inhibitory activity against WalK was evaluated for different bacterial species (S. aureus, E. faecalis, B. subtilis, and S. mutans), and IC 50 values ranging from 37-62 µM were calculated.These results demonstrated that the WalK dimerization domain could serve as a potent binding site, and further optimization of singermycin B could lead to the development of novel antibacterial agents [40].
antibacterial activity against S. epidermidis and S. aureus, including clinical methic sistant S. epidermis (MRSE) and MRSA, which were dramatically improved comp 13a [35].In 2012, Watanabe et al. screened more than 10,000 Streptomyces extracts b differential growth assays and identified signermycin B (14) (Figure 15) as a pote pound that interfered with the WalK dimerization domain.Furthermore, its in activity against WalK was evaluated for different bacterial species (S. aureus, E. fa subtilis, and S. mutans), and IC50 values ranging from 37-62 µM were calculated results demonstrated that the WalK dimerization domain could serve as a potent site, and further optimization of singermycin B could lead to the development o antibacterial agents [40].In another study, Cai et al. in 2011, identified four compounds, 15a-15d (Figure 16), as possible PhoQ inhibitors using HTS and enzymatic activity-coupled assays.These four compounds had significant binding affinities to the S. flexneri PhoQc protein in the surface plasmon resonance (SPR) response and inhibited the autophosphorylation activity of S. flexneri PhoQc (KD = 4.50, 10.6, 7.56, and 9.40 µM, respectively).The IC 50 values of these four compounds calculated during the luminescent kinase assay were 69.37 (15a), 48.9 (15b), 7.99 (15c), and 27.2 (15d) µM.The results showed that all four putative PhoQ inhibitors were able to reduce Shigella virulence [56].
Antibiotics 2024, 13, x FOR PEER REVIEW 12 of 18 flexneri PhoQc (KD = 4.50, 10.6, 7.56, and 9.40 µM, respectively).The IC50 values of these four compounds calculated during the luminescent kinase assay were 69.37 (15a), 48.9 (15b), 7.99 (15c), and 27.2 (15d) µM.The results showed that all four putative PhoQ inhibitors were able to reduce Shigella virulence [56].In 2010, to identify potent inhibitors of BHK, Henriksen et al. performed virtual screening of a library containing approximately 106 compounds.Forty-nine compounds were found to exhibit potent inhibitory activity, and among them, eighteen compounds were directly evaluated against three different S. aureus strains and two E. coli strains via disk inhibition assays.Compounds 17a and 17b (Figure 18) were the most potent, with Gscore values of −7.70 and −7.68 kcal/mol, respectively, and MM-GBSA values of −20.34 and −20.53 kcal/mol, respectively.These compounds can be further optimized for the development of future antibacterial agents [57].four compounds calculated during the luminescent kinase assay were (15b), 7.99 (15c), and 27.2 (15d) µM.The results showed that all four puta itors were able to reduce Shigella virulence [56].In 2010, to identify potent inhibitors of BHK, Henriksen et al. pe screening of a library containing approximately 106 compounds.Forty-n were found to exhibit potent inhibitory activity, and among them, eigh were directly evaluated against three different S. aureus strains and two disk inhibition assays.Compounds 17a and 17b (Figure 18) were the mos In 2010, to identify potent inhibitors of BHK, Henriksen et al. performed virtual screening of a library containing approximately 106 compounds.Forty-nine compounds were found to exhibit potent inhibitory activity, and among them, eighteen compounds were directly evaluated against three different S. aureus strains and two E. coli strains via disk inhibition assays.Compounds 17a and 17b (Figure 18) were the most potent, with G-score values of −7.70 and −7.68 kcal/mol, respectively, and MM-GBSA values of −20.34 and −20.53 kcal/mol, respectively.These compounds can be further optimized for the development of future antibacterial agents [57].In 2010, Okada et al. screened approximately 1368 cultures of Streptomyces sp using differential growth assays and produced different walkmycin derivatives.Am these, walkmycin B (18) (Figure 17) had the greatest binding affinity for WalK in B. sub with a KD value of 7.63 µM.Furthermore, they measured the autophosphorylation ba densitometrically and calculated the IC50 values of 18 against WalK of S. aureus (5.7 and B. subtilis (1.6 µM) [38].
In   In 2010, Okada et al. screened approximately 1368 cultures of Streptomyces sp. by using differential growth assays and produced different walkmycin derivatives.Among these, walkmycin B (18) (Figure 17) had the greatest binding affinity for WalK in B. subtilis, with a KD value of 7.63 µM.Furthermore, they measured the autophosphorylation bands densitometrically and calculated the IC50 values of 18 against WalK of S. aureus (5.7 µM) and B. subtilis (1.6 µM) [38].
In another study, Pan et al. ( 2010) designed and created a series of new 2-arylimino-3-aryl-thiazolidine-4-one compounds based on the core structure of compound 13a (Figure 14) to develop more potent and less harmful BHK inhibitors.Six derivatives (19a-19f) (Figure 19) were created by altering the functional groups through cyclization, aldol condensation, substitution, and hydrolysis.The autophosphorylation activity of WalK was inhibited by all six derivatives in a concentration-dependent manner, with IC50 values that are comparable to those of 13a (IC50 = 47.9 µM) at 88.35, 61.15, 34.83, 66.68, 22.15, and 82.51 µM [58].In 2006, Qin et al. initially employed a structure-based virtual screening (SBVS) method to identify potential inhibitors of S. epidermidis WalK from a small-molecule library of chemical compounds.Among the 76 candidates that target the WalK ATP binding domain, only seven exhibited significant growth-inhibitory effects on S. epidermidis.Compounds 13a and 20a-20b (Figure 20), which possess a thiazolidione scaffold, exhibited greater ATPase activity of the WalK protein, with IC50s ranging from 6.5 to 29 µM.Only the non-biofilm-forming S. epidermidis ATCC 12228 was susceptible to 20b, while 13a and 20a were effective against S. aureus, S. pyogenes, and S. mutans [33].In 2006, Qin et al. initially employed a structure-based virtual screening (SBVS) method to identify potential inhibitors of S. epidermidis WalK from a small-molecule library of chemical compounds.Among the 76 candidates that target the WalK ATP binding domain, only seven exhibited significant growth-inhibitory effects on S. epidermidis.Compounds 13a and 20a-20b (Figure 20), which possess a thiazolidione scaffold, exhibited greater ATPase activity of the WalK protein, with IC 50 s ranging from 6.5 to 29 µM.Only the non-biofilmforming S. epidermidis ATCC 12228 was susceptible to 20b, while 13a and 20a were effective against S. aureus, S. pyogenes, and S. mutans [33].a novel class of competitive ATP inhibitors of BHKs and analyzed its antibacterial act by using the HTVS of compound libraries.The results indicated that 21 has a core structure that is similar to that of purines, although the exact structural mechanism which TEP inhibits BHKs is yet unknown.However, its hydrophobic portion may b sponsible for cell wall permeation, thereby inhibiting bacterial growth.Competitive inhibition was evaluated using Lineweaver-Burk analysis, and the average Ki valu 21 was found to be 0.62 ± 0.11 µM.Furthermore, 21 could serve as a starting materia novel inhibitors that specifically inhibit BHKs [37].22).Prompted by the inhibitory activi imidazoles against BHK, the authors screened imidazole derivatives against the autop phorylation of YycG.Astonishing results were observed for the derivatives, with IC50 ues ranging from 6.6 to 120 µM.Almost 100 zerumbone derivatives were screened their ability to inhibit YycG autophosphorylation.However, the results were not pos and no inhibitor was detected during the study.Then, the authors tried to synth zerumbone derivatives by cleaving their cyclic structures.Upon structural modifica the obtained zerumbone derivatives were found to be active (IC50: 750-2300 µM).Th rivative 29 h was found to be a more potent inhibitor of YycG, with an IC50 value o µM [32].21) as a novel class of competitive ATP inhibitors of BHKs and analyzed its antibacterial activity by using the HTVS of compound libraries.The results indicated that 21 has a core ring structure that is similar to that of purines, although the exact structural mechanism by which TEP inhibits BHKs is yet unknown.However, its hydrophobic portion may be responsible for cell wall permeation, thereby inhibiting bacterial growth.Competitive ATP inhibition was evaluated using Lineweaver-Burk analysis, and the average Ki value for 21 was found to be 0.62 ± 0.11 µM.Furthermore, 21 could serve as a starting material for novel inhibitors that specifically inhibit BHKs [37].21) (Fi a novel class of competitive ATP inhibitors of BHKs and analyzed its antibacter by using the HTVS of compound libraries.The results indicated that 21 has structure that is similar to that of purines, although the exact structural mec which TEP inhibits BHKs is yet unknown.However, its hydrophobic portion sponsible for cell wall permeation, thereby inhibiting bacterial growth.Compe inhibition was evaluated using Lineweaver-Burk analysis, and the average K 21 was found to be 0.62 ± 0.11 µM.Furthermore, 21 could serve as a starting m novel inhibitors that specifically inhibit BHKs [37].22).Prompted by the inhibitory imidazoles against BHK, the authors screened imidazole derivatives against the phorylation of YycG.Astonishing results were observed for the derivatives, wi ues ranging from 6.6 to 120 µM.Almost 100 zerumbone derivatives were sc their ability to inhibit YycG autophosphorylation.However, the results were no and no inhibitor was detected during the study.Then, the authors tried to zerumbone derivatives by cleaving their cyclic structures.Upon structural mo the obtained zerumbone derivatives were found to be active (IC50: 750-2300 µM rivative 29 h was found to be a more potent inhibitor of YycG, with an IC50 v µM [32].22).Prompted by the inhibitory activity of imidazoles against BHK, the authors screened imidazole derivatives against the autophosphorylation of YycG.Astonishing results were observed for the derivatives, with IC 50 values ranging from 6.6 to 120 µM.Almost 100 zerumbone derivatives were screened for their ability to inhibit YycG autophosphorylation.However, the results were not positive, and no inhibitor was detected during the study.Then, the authors tried to synthesize zerumbone derivatives by cleaving their cyclic structures.Upon structural modification, the obtained zerumbone derivatives were found to be active (IC 50 : 750-2300 µM).The derivative 29 h was found to be a more potent inhibitor of YycG, with an IC 50 value of 750 µM [32].In 1993, Roychoudhury et al. identified compounds that prevent the phosphorylation or dephosphorylation of AlgR2 and the DNA-binding activity of AlgR1, which prevent the production of the alginate gene.In this study, 15 compounds were shown to be effective in screening approximately 25,000 compounds for the inhibition of algD promoter activation.Furthermore, four (23a-23d) (Figure 23) of fifteen compounds strongly inhibited AlgR1-AlgR2 phosphorylation, AlgR2 kinase activity, AlgR2 phosphatase activity, the DNA-binding activity of AlgR1, and the kinase activities of CheA, NRⅡ, and KinA [41].

Conclusions
In the present review, we described the roles of the TCS pathway and BHK in bacterial survival and AMR.Furthermore, we also summarize the advancements in the discovery of novel BHK inhibitors in the 21st century.However, despite these massive efforts, none of the discovered inhibitors have entered clinical use or are, to the best of our knowledge, even undergoing clinical studies.To make progress and eventually find new effective antimicrobial medications, challenges must be recognized and overcome.We will use this conclusion section to predict and discuss these possible challenges and obstacles.
Although the chemical structures of the reported inhibitors are diverse, their exact structure-activity relationships cannot be elucidated.Furthermore, progress in the discovery of BHK inhibitors is still in its infancy.Although crystal structures are available, In 1993, Roychoudhury et al. identified compounds that prevent the phosphorylation or dephosphorylation of AlgR2 and the DNA-binding activity of AlgR1, which prevent the production of the alginate gene.In this study, 15 compounds were shown to be effective in screening approximately 25,000 compounds for the inhibition of algD promoter activation.Furthermore, four (23a-23d) (Figure 23) of fifteen compounds strongly inhibited AlgR1-AlgR2 phosphorylation, AlgR2 kinase activity, AlgR2 phosphatase activity, the DNA-binding activity of AlgR1, and the kinase activities of CheA, NRII, and KinA [41].In 1993, Roychoudhury et al. identified compounds that prevent the phosphorylation or dephosphorylation of AlgR2 and the DNA-binding activity of AlgR1, which prevent the production of the alginate gene.In this study, 15 compounds were shown to be effective in screening approximately 25,000 compounds for the inhibition of algD promoter activation.Furthermore, four (23a-23d) (Figure 23) of fifteen compounds strongly inhibited AlgR1-AlgR2 phosphorylation, AlgR2 kinase activity, AlgR2 phosphatase activity, the DNA-binding activity of AlgR1, and the kinase activities of CheA, NRⅡ, and KinA [41].

Conclusions
In the present review, we described the roles of the TCS pathway and BHK in bacterial survival and AMR.Furthermore, we also summarize the advancements in the discovery of novel BHK inhibitors in the 21st century.However, despite these massive efforts, none of the discovered inhibitors have entered clinical use or are, to the best of our knowledge, even undergoing clinical studies.To make progress and eventually find new effective antimicrobial medications, challenges must be recognized and overcome.We will use this conclusion section to predict and discuss these possible challenges and obstacles.
Although the chemical structures of the reported inhibitors are diverse, their exact structure-activity relationships cannot be elucidated.Furthermore, progress in the discovery of BHK inhibitors is still in its infancy.Although crystal structures are available, the lack of cocrystals makes it cumbersome to identify potential receptor-ligand interactions.Some studies based on fragment-based and structure-based virtual screening and drug repositioning were implemented to identify BHK inhibitors that exhibited significant inhibitory potential.In the near future, understanding the binding mode and conducting molecular modeling studies will significantly accelerate the discovery of novel

Conclusions
In the present review, we described the roles of the TCS pathway and BHK in bacterial survival and AMR.Furthermore, we also summarize the advancements in the discovery of novel BHK inhibitors in the 21st century.However, despite these massive efforts, none of the discovered inhibitors have entered clinical use or are, to the best of our knowledge, even undergoing clinical studies.To make progress and eventually find new effective antimicrobial medications, challenges must be recognized and overcome.We will use this conclusion section to predict and discuss these possible challenges and obstacles.
Although the chemical structures of the reported inhibitors are diverse, their exact structure-activity relationships cannot be elucidated.Furthermore, progress in the discovery of BHK inhibitors is still in its infancy.Although crystal structures are available, the lack of cocrystals makes it cumbersome to identify potential receptor-ligand interactions.Some studies based on fragment-based and structure-based virtual screening and drug repositioning were implemented to identify BHK inhibitors that exhibited significant inhibitory potential.In the near future, understanding the binding mode and conducting molecular modeling studies will significantly accelerate the discovery of novel BHK inhibitors with greater potency.In addition, researchers can perform more prospective analyses by inducing spontaneous mutants to BHK inhibitors that are under development to elucidate on-target effects and possible resistance mechanisms.Although challenging, designing and developing novel BHK inhibitors is a viable approach for combating AMR.

Figure 1 .
Figure 1.The TCS signaling pathway and role of bacterial histidine kinase in gene regulation.DHp domain-Dimerization and histidine phosphotransfer domain; C A domain-Catalytic and ATP binding domain; H-box-Highly conserved histidine residue; P-Phosphoryl group.

Figure 1 .
Figure 1.The TCS signaling pathway and role of bacterial histidine kinase in gene regulation.DHp domain-Dimerization and histidine phosphotransfer domain; C A domain-Catalytic and ATP binding domain; H-box-Highly conserved histidine residue; P-Phosphoryl group.

Figure 8 .
Figure 8.Chemical structures of diaryl pyrazole-based derivatives 7a-7d.In 2017, Zheng et al. used whole-cell phenotypic high-throughput screening to screen a small-molecule library of approximately 540,000 compounds to identify new DosRST inhibitors.Compounds 8a and 8b (Figure9) were identified as potential antibacterial agents.Compound 8a reduced the autophosphorylation of DosS with an IC 50 of 1.9 µM, and 8b inhibited the autophosphorylation of both DosS and DosT with IC 50 s of 0.5 and 5 µM, respectively[53].

Figure 12 .
Figure 12.Chemical structures of adenine derivatives 11a-11i.In 2014, Bellale et al. discovered a particular class of diarylthiazole compounds (Figure13) that had potent inhibitory activity against PrrBA TCA, which is required for the viability of M. tuberculosis.Over 40 diarylthiazole derivatives, such as 12a and 12b, which demonstrated remarkable antibacterial activities with MICs of 0.4 and 0.25 µg/ml, respectively, were subsequently developed, and the majority of these derivatives exhibited favorable physicochemical characteristics and significant MICs against M. tuberculosis (MIC ≤1 µg/mL)[55].

Figure 13 .
Figure 13.Chemical structures of diarylthiazole derivatives 12a-12b.In another study by Liu et al. in 2014, six analogs of thiazolidine (13a) (13b-13g) (Figure 14) were developed and created by altering functional groups to enhance the antibacterial activity and decrease the toxicity of 13a.The results indicated the inhibitory effects of these compounds on the autophosphorylation of WalK, with IC50 values ranging from 24.2 to 71.2 µM.With MICs ranging from 1.5 to 6.3 µM, these compounds exhibited strong

Figure 13 .
Figure 13.Chemical structures of diarylthiazole derivatives 12a-12b.In another study by Liu et al. in 2014, six analogs of thiazolidine (13a) (13b-13g) (Figure 14) were developed and created by altering functional groups to enhance the antibacterial activity and decrease the toxicity of 13a.The results indicated the inhibitory effects of these compounds on the autophosphorylation of WalK, with IC50 values ranging from 24.2 to 71.2 µM.With MICs ranging from 1.5 to 6.3 µM, these compounds exhibited strong

Figure 13 .Figure 14 .
Figure 13.Chemical structures of diarylthiazole derivatives 12a-12b.In another study by Liu et al. in 2014, six analogs of thiazolidine (13a) (13b-13g) (Figure 14) were developed and created by altering functional groups to enhance the antibacterial activity and decrease the toxicity of 13a.The results indicated the inhibitory effects of these compounds on the autophosphorylation of WalK, with IC 50 values ranging from 24.2 to 71.2 µM.With MICs ranging from 1.5 to 6.3 µM, these compounds exhibited

Figure 16 .
Figure 16.Chemical structures of PhoQ inhibitors 15a-15d.Another study by Eguchi et al. in 2011 investigated the effect of walkmycin C (16) (Figure 17) on WalK BHK in B. subtilis and S. aureus.Furthermore, walkmycin also exhibited significant activity against the cytoplasmic domains of VicK (IC50: 2.53 µg/ml), CiaH (IC50: 4.29 µg/ml), and LiaS (IC50: 4.96 µg/ml) of Streptococcus mutans.Moreover, it also inhibited the autophosphorylation activities of EnvZ and PhoQ from E. coli, both with IC50s of 1.25 µM.Studies of the inhibitory activity of walkmycin C on the virulence factors of S. mutans showed that exposure to walkmycin C at sub-MICs could inhibit biofilm formation, acid tolerance, and competence.Thus, walkmycin C can be used as a potential lead molecule for the development of BHK inhibitors [39].

Figure 16 .
Figure 16.Chemical structures of PhoQ inhibitors 15a-15d.Another study by Eguchi et al. in 2011 investigated the effect of walkmycin C (16) (Figure 17) on WalK BHK in B. subtilis and S. aureus.Furthermore, walkmycin also exhibited significant activity against the cytoplasmic domains of VicK (IC50: 2.53 µg/mL), CiaH (IC50: 4.29 µg/mL), and LiaS (IC 50 : 4.96 µg/mL) of Streptococcus mutans.Moreover, it also inhibited the autophosphorylation activities of EnvZ and PhoQ from E. coli, both with IC 50 s of 1.25 µM.Studies of the inhibitory activity of walkmycin C on the virulence factors of S. mutans showed that exposure to walkmycin C at sub-MICs could inhibit biofilm formation, acid tolerance, and competence.Thus, walkmycin C can be used as a potential lead molecule for the development of BHK inhibitors [39].
another study, Pan et al. (2010) designed and created a series of new 2-arylim 3-aryl-thiazolidine-4-one compounds based on the core structure of compound 13a ( ure 14) to develop more potent and less harmful BHK inhibitors.Six derivatives (19a-(Figure 19) were created by altering the functional groups through cyclization, aldol densation, substitution, and hydrolysis.The autophosphorylation activity of WalK inhibited by all six derivatives in a concentration-dependent manner, with IC50 values are comparable to those of 13a (IC50 = 47.9 µM) at 88.35, 61.15, 34.83, 66.68, 22.15, and 8 µM [58].

Figure 18 . 18 Figure 18 .
Figure 18.Chemical structures of BHK inhibitors 17a-17b.In 2010, Okada et al. screened approximately 1368 cultures of Streptomyces sp. by using differential growth assays and produced different walkmycin derivatives.Among these, walkmycin B (18) (Figure17) had the greatest binding affinity for WalK in B. subtilis, with a K D value of 7.63 µM.Furthermore, they measured the autophosphorylation bands densitometrically and calculated the IC 50 values of 18 against WalK of S. aureus (5.7 µM) and B. subtilis (1.6 µM)[38].In another study, Pan et al. (2010) designed and created a series of new 2-arylimino-3aryl-thiazolidine-4-one compounds based on the core structure of compound 13a (Figure14) to develop more potent and less harmful BHK inhibitors.Six derivatives (19a-19f) (Figure19) were created by altering the functional groups through cyclization, aldol condensation, substitution, and hydrolysis.The autophosphorylation activity of WalK was inhibited by all six derivatives in a concentration-dependent manner, with IC 50 values that are comparable to those of 13a (IC 50 = 47.9 µM) at 88.35, 61.15, 34.83, 66.68, 22.15, and 82.51 µM[58].

Figure 20 .
Figure 20.Chemical structures of compounds 20a-20b.Gilmour et al. (2005) identified thienopyridine (CAS 332175-01-6) (21) (Figure 2a novel class of competitive ATP inhibitors of BHKs and analyzed its antibacterial act by using the HTVS of compound libraries.The results indicated that 21 has a core structure that is similar to that of purines, although the exact structural mechanism which TEP inhibits BHKs is yet unknown.However, its hydrophobic portion may b sponsible for cell wall permeation, thereby inhibiting bacterial growth.Competitive inhibition was evaluated using Lineweaver-Burk analysis, and the average Ki valu 21 was found to be 0.62 ± 0.11 µM.Furthermore, 21 could serve as a starting materia novel inhibitors that specifically inhibit BHKs[37].

Figure 21 .
Figure 21.Chemical structure of thienopyridine (21).In 2001, Yamamoto et al. developed and examined a series of imidazole (22aand zerumbone (22f-22k) derivatives (Figure22).Prompted by the inhibitory activi imidazoles against BHK, the authors screened imidazole derivatives against the autop phorylation of YycG.Astonishing results were observed for the derivatives, with IC50 ues ranging from 6.6 to 120 µM.Almost 100 zerumbone derivatives were screened their ability to inhibit YycG autophosphorylation.However, the results were not pos and no inhibitor was detected during the study.Then, the authors tried to synth zerumbone derivatives by cleaving their cyclic structures.Upon structural modifica the obtained zerumbone derivatives were found to be active (IC50: 750-2300 µM).Th rivative 29 h was found to be a more potent inhibitor of YycG, with an IC50 value o µM[32].

Figure 20 .
Figure 20.Chemical structures of compounds 20a-20b.Gilmour et al. (2005) identified thienopyridine (CAS 332175-01-6) (21) (Figure21) as a novel class of competitive ATP inhibitors of BHKs and analyzed its antibacterial activity by using the HTVS of compound libraries.The results indicated that 21 has a core ring structure that is similar to that of purines, although the exact structural mechanism by which TEP inhibits BHKs is yet unknown.However, its hydrophobic portion may be responsible for cell wall permeation, thereby inhibiting bacterial growth.Competitive ATP inhibition was evaluated using Lineweaver-Burk analysis, and the average Ki value for 21 was found to be 0.62 ± 0.11 µM.Furthermore, 21 could serve as a starting material for novel inhibitors that specifically inhibit BHKs[37].

Figure 21 .
Figure 21.Chemical structure of thienopyridine (21).In 2001, Yamamoto et al. developed and examined a series of imidazole (22a-22e) and zerumbone (22f-22k) derivatives (Figure22).Prompted by the inhibitory activity of imidazoles against BHK, the authors screened imidazole derivatives against the autophosphorylation of YycG.Astonishing results were observed for the derivatives, with IC 50 values ranging from 6.6 to 120 µM.Almost 100 zerumbone derivatives were screened for their ability to inhibit YycG autophosphorylation.However, the results were not positive, and no inhibitor was detected during the study.Then, the authors tried to synthesize zerumbone derivatives by cleaving their cyclic structures.Upon structural modification, the obtained zerumbone derivatives were found to be active (IC 50 : 750-2300 µM).The derivative 29 h was found to be a more potent inhibitor of YycG, with an IC 50 value of 750 µM[32].

Table 1 .
BHK and its inhibitors.