Tue. Dec 24th, 2024

Se (Promega, Madison, WI). One ml of each reverse transcriptase reaction was used as a template in a PCR reaction containing the following specific primer pairs: Cyclophilin (at2g36130) AGTCCGCCGGAGGTTACGCT (as normalizer) and TGGATCGGCCTGTCGGTGTT and for EHD1 GGGGATCCATGGAGATCGAATCCGTCGC and CTGCTTGAACTGCTACTGTG. To monitor the expression of EHD1 forms in the transgenic plants a 4ul aliquot of each reverse transcriptase reaction was used as template in a PCR reaction containing the following primers EHD1-DCC(2) FOR (TTTGGAAAGGTACAAAGAG) and GFP REV (GGGCCAGGGCACGGGCAGCTT). The amplified FD&C Yellow 5 fragment was 370 bp long. Quantification of the resultant PCR reactions was performed using ImageJ software.and EHD2 knock-down seedlings. 7?0 day old transgenic seedlings were floated on a 200 mM NaCl solution for 60 minutes or a 50 mM BFA solution for 30 minutes, both supplemented with 5 mM Fm-4-64, and then washed. Root sections were visualized under a laser-scanning confocal microscope. Scale bar = 10 mm. (TIF)Figure S3 Expression of EHD1 forms in transgenicArabidopsis plants. cDNA was prepared from 5? day old transgenic seedlings as indicated. The presence of the GFP tagged EHD1/DEH/DCC cDNA was confirmed by PCR. (TIF)AcknowledgmentsWe thank Prof. N. Geldner for providing the Arabidopsis wave lines and wave markers.ROS quantificationROS were quantified as described in [47]. Roots of 1 week old Arabiopsis seedlings were floated on a 200 mM NaCl solution for 18325633 2 hours, then washed and stained with AmplexH Red (Invitrogen).Author ContributionsConceived and Sudan I custom synthesis designed the experiments: MB AA. Performed the experiments: MB ML SS HP. Analyzed the data: MB AA. Wrote the paper: MB AA.
The reemergence of infectious diseases and the continuous development of antimicrobial drug resistance in pathogens have been causing an alarming deficit in effective antibacterial agents, leading to a growing threat to public healthcare worldwide. Extended-spectrum b-lactamase (ESBL)-producing Enterobacteriaceae have become the most frequent nosocomial pathogens and have posed serious challenges to clinicians because of their resistance to many classes of antibiotics [1]. ESBLs are the enzymes produced by Gram-negative bacteria that mediate resistance to third-generation cephalosporins (such as cefotaxime and ceftriaxone) by hydrolysis of these antibiotics [2]. Plasmidmediated ESBL enzymes are of special interest in the generation of ESBL variants [3]. Infections caused by Enterobacteriaceae producing ESBL often complicate the therapy and limit treatmentoptions, often necessitating combination therapy [4]. Combinations of a b-lactam with either a b-lactamase inhibitor or a fluoroquinolone, or double b-lactam combinations are common, but these may not always prevent the emergence of resistance [4], [5]. Several reviews recently emphasized the urgent need 16402044 for new therapeutic strategies [6], [7]. (2)-Epigallocatechin-3-gallate (EGCG), a main constituent of green tea polyphenol, has been reported to have great antiinfective potential [8], [9] and also aids other antibiotics against both antibiotic-resistant Gram-positive [10], [11] and Gramnegative bacteria [12], [13] at sub-minimum inhibitory concentrations (sub-MICs). Synergy between EGCG and b-lactam against b-lactamase producing Staphylococcus aureus can be easily explained by the fact that both antibacterial compounds attack the same site of the peptidoglycan layer in Gram-positive bacteria [11], [14]. Since EGCG is not able to b.Se (Promega, Madison, WI). One ml of each reverse transcriptase reaction was used as a template in a PCR reaction containing the following specific primer pairs: Cyclophilin (at2g36130) AGTCCGCCGGAGGTTACGCT (as normalizer) and TGGATCGGCCTGTCGGTGTT and for EHD1 GGGGATCCATGGAGATCGAATCCGTCGC and CTGCTTGAACTGCTACTGTG. To monitor the expression of EHD1 forms in the transgenic plants a 4ul aliquot of each reverse transcriptase reaction was used as template in a PCR reaction containing the following primers EHD1-DCC(2) FOR (TTTGGAAAGGTACAAAGAG) and GFP REV (GGGCCAGGGCACGGGCAGCTT). The amplified fragment was 370 bp long. Quantification of the resultant PCR reactions was performed using ImageJ software.and EHD2 knock-down seedlings. 7?0 day old transgenic seedlings were floated on a 200 mM NaCl solution for 60 minutes or a 50 mM BFA solution for 30 minutes, both supplemented with 5 mM Fm-4-64, and then washed. Root sections were visualized under a laser-scanning confocal microscope. Scale bar = 10 mm. (TIF)Figure S3 Expression of EHD1 forms in transgenicArabidopsis plants. cDNA was prepared from 5? day old transgenic seedlings as indicated. The presence of the GFP tagged EHD1/DEH/DCC cDNA was confirmed by PCR. (TIF)AcknowledgmentsWe thank Prof. N. Geldner for providing the Arabidopsis wave lines and wave markers.ROS quantificationROS were quantified as described in [47]. Roots of 1 week old Arabiopsis seedlings were floated on a 200 mM NaCl solution for 18325633 2 hours, then washed and stained with AmplexH Red (Invitrogen).Author ContributionsConceived and designed the experiments: MB AA. Performed the experiments: MB ML SS HP. Analyzed the data: MB AA. Wrote the paper: MB AA.
The reemergence of infectious diseases and the continuous development of antimicrobial drug resistance in pathogens have been causing an alarming deficit in effective antibacterial agents, leading to a growing threat to public healthcare worldwide. Extended-spectrum b-lactamase (ESBL)-producing Enterobacteriaceae have become the most frequent nosocomial pathogens and have posed serious challenges to clinicians because of their resistance to many classes of antibiotics [1]. ESBLs are the enzymes produced by Gram-negative bacteria that mediate resistance to third-generation cephalosporins (such as cefotaxime and ceftriaxone) by hydrolysis of these antibiotics [2]. Plasmidmediated ESBL enzymes are of special interest in the generation of ESBL variants [3]. Infections caused by Enterobacteriaceae producing ESBL often complicate the therapy and limit treatmentoptions, often necessitating combination therapy [4]. Combinations of a b-lactam with either a b-lactamase inhibitor or a fluoroquinolone, or double b-lactam combinations are common, but these may not always prevent the emergence of resistance [4], [5]. Several reviews recently emphasized the urgent need 16402044 for new therapeutic strategies [6], [7]. (2)-Epigallocatechin-3-gallate (EGCG), a main constituent of green tea polyphenol, has been reported to have great antiinfective potential [8], [9] and also aids other antibiotics against both antibiotic-resistant Gram-positive [10], [11] and Gramnegative bacteria [12], [13] at sub-minimum inhibitory concentrations (sub-MICs). Synergy between EGCG and b-lactam against b-lactamase producing Staphylococcus aureus can be easily explained by the fact that both antibacterial compounds attack the same site of the peptidoglycan layer in Gram-positive bacteria [11], [14]. Since EGCG is not able to b.