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BioSpec cems linked to the

a PA01 biofilms were cultivated in the <t>combined</t> <t>CEMS-BioSpec</t> system with 10 g L −1 TSB supplied at a flow rate of 12.5 mL h −1 . Changes in biofilm metabolic activity (black line) and biofilm biomass (magenta line) were monitored in real-time over the course of 125 h. Total protein from biofilm biomass (red dashed line) was sampled eight times during the first 75 h, each point is the mean of biological duplicates, technical triplicates with the standard deviation indicated by the error bar ( n = 6). b Direct correlation of total protein isolated from the sessile biomass with the corresponding BioSpec absorbance measurements of attached biomass ( r = 0.96, r 2 = 0.92, p < 0.05). Simple linear correlation was performed with Pearson correlation coefficient ( r ) and coefficient of determination ( R 2 ) calculated for each correlation.

Cems Linked To The, supplied by BioSpec, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/cems linked to the/product/BioSpec
Average 90 stars, based on 1 article reviews

cems linked to the - by Bioz Stars, 2026-05

90/100 stars

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1) Product Images from "Biofilm dynamics: linking in situ biofilm biomass and metabolic activity measurements in real-time under continuous flow conditions"

Article Title: Biofilm dynamics: linking in situ biofilm biomass and metabolic activity measurements in real-time under continuous flow conditions

Journal: NPJ Biofilms and Microbiomes

doi: 10.1038/s41522-020-00153-9

a PA01 biofilms were cultivated in the combined CEMS-BioSpec system with 10 g L −1 TSB supplied at a flow rate of 12.5 mL h −1 . Changes in biofilm metabolic activity (black line) and biofilm biomass (magenta line) were monitored in real-time over the course of 125 h. Total protein from biofilm biomass (red dashed line) was sampled eight times during the first 75 h, each point is the mean of biological duplicates, technical triplicates with the standard deviation indicated by the error bar ( n = 6). b Direct correlation of total protein isolated from the sessile biomass with the corresponding BioSpec absorbance measurements of attached biomass ( r = 0.96, r 2 = 0.92, p < 0.05). Simple linear correlation was performed with Pearson correlation coefficient ( r ) and coefficient of determination ( R 2 ) calculated for each correlation.

Figure Legend Snippet: a PA01 biofilms were cultivated in the combined CEMS-BioSpec system with 10 g L −1 TSB supplied at a flow rate of 12.5 mL h −1 . Changes in biofilm metabolic activity (black line) and biofilm biomass (magenta line) were monitored in real-time over the course of 125 h. Total protein from biofilm biomass (red dashed line) was sampled eight times during the first 75 h, each point is the mean of biological duplicates, technical triplicates with the standard deviation indicated by the error bar ( n = 6). b Direct correlation of total protein isolated from the sessile biomass with the corresponding BioSpec absorbance measurements of attached biomass ( r = 0.96, r 2 = 0.92, p < 0.05). Simple linear correlation was performed with Pearson correlation coefficient ( r ) and coefficient of determination ( R 2 ) calculated for each correlation.

Techniques Used: Activity Assay, Standard Deviation, Isolation

P. aeruginosa PAO1 biofilms were cultivated under flow with a nutrient concentration of 3 g L −1 TSB until whole-biofilm metabolic activity (black line) and approximate biomass (magenta line) steady-state was reached (0 ± 70 h) ( a ). The inflow of nutrient solution was replaced with a solution of diluted sodium hypochlorite diluted with dH 2 O (1:100, 570 ppm free chlorine). The sodium hypochlorite solution was aseptically introduced into the system using the same flow rate for a treatment period of 1 h (green shaded region) followed by reintroduction of nutrient medium (recovery phase, post 71 h). b Zoomed-in view showing a 15 h period spanning pre-perturbation and recovery phase. The free chlorine concentrations in the effluent from the CEMS-BioSpec system (red line) was determine prior to the start of the treatment period, during and for 1 h after the treatment period (±70–71 h). Error bars of all free chlorine data points represent the standard error of triplicate readings at each time point ( n = 3).

Figure Legend Snippet: P. aeruginosa PAO1 biofilms were cultivated under flow with a nutrient concentration of 3 g L −1 TSB until whole-biofilm metabolic activity (black line) and approximate biomass (magenta line) steady-state was reached (0 ± 70 h) ( a ). The inflow of nutrient solution was replaced with a solution of diluted sodium hypochlorite diluted with dH 2 O (1:100, 570 ppm free chlorine). The sodium hypochlorite solution was aseptically introduced into the system using the same flow rate for a treatment period of 1 h (green shaded region) followed by reintroduction of nutrient medium (recovery phase, post 71 h). b Zoomed-in view showing a 15 h period spanning pre-perturbation and recovery phase. The free chlorine concentrations in the effluent from the CEMS-BioSpec system (red line) was determine prior to the start of the treatment period, during and for 1 h after the treatment period (±70–71 h). Error bars of all free chlorine data points represent the standard error of triplicate readings at each time point ( n = 3).

Techniques Used: Concentration Assay, Activity Assay

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Image Search Results

Journal: NPJ Biofilms and Microbiomes

Article Title: Biofilm dynamics: linking in situ biofilm biomass and metabolic activity measurements in real-time under continuous flow conditions

doi: 10.1038/s41522-020-00153-9

Figure Lengend Snippet: a PA01 biofilms were cultivated in the combined CEMS-BioSpec system with 10 g L −1 TSB supplied at a flow rate of 12.5 mL h −1 . Changes in biofilm metabolic activity (black line) and biofilm biomass (magenta line) were monitored in real-time over the course of 125 h. Total protein from biofilm biomass (red dashed line) was sampled eight times during the first 75 h, each point is the mean of biological duplicates, technical triplicates with the standard deviation indicated by the error bar ( n = 6). b Direct correlation of total protein isolated from the sessile biomass with the corresponding BioSpec absorbance measurements of attached biomass ( r = 0.96, r 2 = 0.92, p < 0.05). Simple linear correlation was performed with Pearson correlation coefficient ( r ) and coefficient of determination ( R 2 ) calculated for each correlation.

Article Snippet: Sessile growth dynamics were studied under continuous flow conditions within the CEMS linked to the BioSpec, allowing for the simultaneous real time, nondestructive monitoring of biofilm metabolism, and biomass respectively (Fig. ).

Techniques: Activity Assay, Standard Deviation, Isolation

Journal: NPJ Biofilms and Microbiomes

Article Title: Biofilm dynamics: linking in situ biofilm biomass and metabolic activity measurements in real-time under continuous flow conditions

doi: 10.1038/s41522-020-00153-9

Figure Lengend Snippet: P. aeruginosa PAO1 biofilms were cultivated under flow with a nutrient concentration of 3 g L −1 TSB until whole-biofilm metabolic activity (black line) and approximate biomass (magenta line) steady-state was reached (0 ± 70 h) ( a ). The inflow of nutrient solution was replaced with a solution of diluted sodium hypochlorite diluted with dH 2 O (1:100, 570 ppm free chlorine). The sodium hypochlorite solution was aseptically introduced into the system using the same flow rate for a treatment period of 1 h (green shaded region) followed by reintroduction of nutrient medium (recovery phase, post 71 h). b Zoomed-in view showing a 15 h period spanning pre-perturbation and recovery phase. The free chlorine concentrations in the effluent from the CEMS-BioSpec system (red line) was determine prior to the start of the treatment period, during and for 1 h after the treatment period (±70–71 h). Error bars of all free chlorine data points represent the standard error of triplicate readings at each time point ( n = 3).

Techniques: Concentration Assay, Activity Assay