We provide the first evidence that the size (diameter) of carbon nanotubes (CNTs) is a key factor governing their antibacterial effects and that the likely main CNT-cytotoxicity mechanism is cell membrane damage by direct contact with CNTs. Experiments with well-characterized single-walled carbon nanotubes (SWNTs) and multiwalled carbon nanotubes (MWNTs) demonstrate that SWNTs are much more toxic to bacteria than MWNTs. Gene expression data show that in the presence of both MWNTs and SWNTs, Escherichia coli expresses high levels of stress-related gene products, with the quantity and magnitude of expression being much higher in the presence of SWNTs.
Eight Escherichia coli strains were studied in minimal medium with a continuous flow system using confocal microscopy. K12 wild-type strains ATCC 25404 and MG1655 formed the best biofilms ( approximately 43 microm thick, 21 to 34% surface coverage). JM109, DH5alpha, and MG1655 motA formed intermediate biofilms ( approximately 13 microm thick, 41 to 58% surface coverage). BW25113, MG1655 qseB, and MG1655 fliA had poor biofilms (surface coverage less than 5%). The best biofilm-formers, ATCC 25404 and MG1655, displayed the highest motility, whereas the worst biofilm former, BW25113, was motility-impaired. The differences in motility were due to differences in expression of the motility loci qseB, flhD, fliA, fliC, and motA (e.g., qseB expression in MG1655 was 139-fold higher than BW25113 and 209-fold higher than JM109). Motility affected the biofilm architecture as those strains which had poor motility (E. coli JM109, E. coli MG1655 motA, and DH5alpha) formed flatter microcolonies compared with MG1655 and ATCC 25404, which had more dramatic vertical structures as a result of their enhanced motility. The presence of flagella was also found to be important as qseB and fliA mutants (which lack flagella) had less biofilm than the isogenic paralyzed motA strain (threefold less thickness and 15-fold less surface coverage).
This study elucidates the mechanisms by which extracellular polymeric substances (EPS) impact permeate water flux and salt rejection during biofouling of reverse osmosis (RO) membranes. RO fouling experiments were conducted with Pseudomonas aeruginosa PAO1, EPS extracted from PAO1 biofilms, and dead PAO1 cells fixed in formaldehyde. While a biofouling layer of dead bacterial cells decreases salt rejection and permeate flux by a biofilm-enhanced osmotic pressure mechanism, the EPS biofouling layer adversely impacts permeate flux by increasing the hydraulic resistance to permeate flow. During controlled fouling experiments with extracted EPS in a simulated wastewater solution, polysaccharides adsorbed on the RO membranes much more effectively than proteins (adsorption efficiencies of 61.2-88.7% and 11.6-12.4% for polysaccharides and proteins, respectively). Controlled fouling experiments with EPS in sodium chloride solutions supplemented with 0.5 mM calcium ions (total ionic strength of 15 mM) indicate that calcium increases the adsorption efficiency of polysaccharides and DNA by 2- and 3-fold, respectively. The increased adsorption of EPS onto the membrane resulted in a significant decrease in permeate water flux. Corroborating with these calcium effects, atomic force microscopy (AFM) measurements demonstrated that addition of calcium ions to the feed solution results in a marked increase in the adhesion forces between a carboxylated particle probe and the EPS layer. The increase in the interfacial adhesion forces is attributed to specific EPS-calcium interactions that play a major role in biofouling of RO membranes.
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