Dataset: Iron concentrations of phage from experiments of iron-labelled E. coli infected with T4 and T5 bacteriophage, 2018 and 2019.

Name: Iron concentrations of phage from experiments of iron-labelled E. coli infected with T4 and T5 bacteriophage, 2018 and 2019.
Published: 2019-02-27
Keywords: biota, oceans

Release Date:2020-01-27Final no updates expectedDOI: 10.1575/1912/bco-dmo.757485.1Version 1 (2019-02-27)Dataset Type:experimental

Principal Investigator: Mya Breitbart (University of South Florida)

Principal Investigator: Kristen Nicolle Buck (University of South Florida)

Co-Principal Investigator: Chelsea Bonnain (University of South Florida)

Co-Principal Investigator: Salvatore Caprara (University of South Florida)

BCO-DMO Data Manager: Nancy Copley (Woods Hole Oceanographic Institution)

Project: EAGER: Iron-Virus Interactions in the Ocean (Fe-Virus)

Abstract

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File(s)	Type	Description	Action
Fe_label_Ecoli_T4_T5.csv (126.12 KB)	Comma Separated Values (.csv)	Primary data file for dataset ID 757485	Download

Supplemental File(s)	Type	Description	Action
Table2.PNG (33.46 KB)	Portable Network Graphics (.png)	Table 2: Analytical blank values for 56Fe and 57Fe after rhodium correction as measured on ELEMENT XR ICP-MS. “Expt” refers to experimental and analytical dataset; e.g. Expt 2.1 is experiment 2, first analytical dataset, while Expt 2.2 is experiment 2, second analytical dataset. The number of blank measurements used to calculate the average and standard deviation for each round is “n”.	Download
Table1.PNG (72.58 KB)	Portable Network Graphics (.png)	Table 1: M9 minimal media composition from Kutter and Sulakvelidze (2004). A 1 L stock of 20X M9 Salts and 0.5 L of all stock solutions were weighed separately in acid-cleaned Nalgene fluorinated HDPE bottles and brought to desired concentrations using Milli-Q water (18.2 MΩ cm). A 1 L volume of liquid culture was prepared by adding all sterile stock solution components to 912.5 mL of Milli-Q water in an acid-cleaned HDPE bottle on a balance. *FeSO4 added as 57FeSO4 spike separately after all other components combined. Completed M9 minimal media was 0.02 µm filtered prior to use.	Download
Figure3.PNG (151.65 KB)	Plain Text	Figure 3: Flowchart of the Tracing 57Fe to E. coli phages T4 & T5 Experimental method. First, cell cultures were grown and aliquoted into triplicate samples of each treatment: T4 infected (A, B, C), T5 infected (M, N, O), Bacterial Control (D, E, F), and Blank Control (G, H, I). Cell cultures were rinsed to remove excess 57Fe, then lysed by phage T4 infection, phage T5 infection, or chloroform for the bacterial lysis control. The lysates are then purified for the phage by centrifugation, filtration, sucrose ultracentrifugation, and dialysis.	Download
Figure2.PNG (129.69 KB)	Portable Network Graphics (.png)	Figure 2: Schematic of E. coli cell preparation	Download
Figure1.PNG (34.65 KB)	Portable Network Graphics (.png)	Growth curve for E. coli ZK126 measured on a spectrophotometer. Mid-logarithmic growth (indicated by shaded area) was an OD600= 0.200-0.500.	Download

This data was collected as part of a study investigating the source of iron to bacteriophage (phage for short, or viruses that infect and kill bacteria) progeny. Evidence from a phage that infects E. coli shows iron incorporated into the tail fiber structure. This study aims at identifying whether the source of the iron is environmental or bacterially derived. E. coli bacterial cultures were grown in minimal media spiked with 10 µM 57FeSO4 then infected with phage T4 or T5. The phages were purified by methods of centrifugation, filtration, density-dependent ultracentrifugation, and dialyzing. The resulting phage fractions were quantified by SYBR epifluorescence microscopy and metal concentrations were measured on an ELEMENT XR ICP-MS.

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Related Publications

Methods

Gledhill, M. (2012). The organic complexation of iron in the marine environment: a review. Frontiers in Microbiology, 3. doi:10.3389/fmicb.2012.00069

Methods

Hurwitz, B. L., Deng, L., Poulos, B. T., & Sullivan, M. B. (2012). Evaluation of methods to concentrate and purify ocean virus communities through comparative, replicated metagenomics. Environmental Microbiology, 15(5), 1428–1440. doi:10.1111/j.1462-2920.2012.02836.x

Methods

Kutter, E., & Sulakvelidze, A. (2004). Bacteriophages: biology and applications. CRC Press.

Methods

Mellett, T., Brown, M.T., Chappell, P.D., Duckham, C., Fitzsimmons, J.N., Till, C.P., Sherrell, R.M., Maldonado, M.T., and Buck, K.N. (2017). The biogeochemical cycling of iron, copper, nickel, cadmium, manganese, cobalt, lead, and scandium in a California Current experimental study. Limnology and Oceanography, 63(S1), S425–S447. doi:10.1002/lno.10751

Methods

Noble, R., & Fuhrman, J. (1998). Use of SYBR Green I for rapid epifluorescence counts of marine viruses and bacteria. Aquatic Microbial Ecology, 14, 113–118. doi:10.3354/ame014113

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Dataset: Iron concentrations of phage from experiments of iron-labelled E. coli infected with T4 and T5 bacteriophage, 2018 and 2019.

Release Date:2020-01-27Final no updates expectedDOI: 10.1575/1912/bco-dmo.757485.1Version 1 (2019-02-27)Dataset Type:experimental

Principal Investigator: Mya Breitbart (University of South Florida)

Principal Investigator: Kristen Nicolle Buck (University of South Florida)

Co-Principal Investigator: Chelsea Bonnain (University of South Florida)

Co-Principal Investigator: Salvatore Caprara (University of South Florida)

BCO-DMO Data Manager: Nancy Copley (Woods Hole Oceanographic Institution)

Project: EAGER: Iron-Virus Interactions in the Ocean (Fe-Virus)

Abstract

Cite Dataset

XXX

Views

XX

Downloads

X

Citations

Download All Add to Cart

File(s)	Type	Description	Action
Fe_label_Ecoli_T4_T5.csv (126.12 KB)	Comma Separated Values (.csv)	Primary data file for dataset ID 757485	Download

Supplemental File(s)	Type	Description	Action
Table2.PNG (33.46 KB)	Portable Network Graphics (.png)	Table 2: Analytical blank values for 56Fe and 57Fe after rhodium correction as measured on ELEMENT XR ICP-MS. “Expt” refers to experimental and analytical dataset; e.g. Expt 2.1 is experiment 2, first analytical dataset, while Expt 2.2 is experiment 2, second analytical dataset. The number of blank measurements used to calculate the average and standard deviation for each round is “n”.	Download
Table1.PNG (72.58 KB)	Portable Network Graphics (.png)	Table 1: M9 minimal media composition from Kutter and Sulakvelidze (2004). A 1 L stock of 20X M9 Salts and 0.5 L of all stock solutions were weighed separately in acid-cleaned Nalgene fluorinated HDPE bottles and brought to desired concentrations using Milli-Q water (18.2 MΩ cm). A 1 L volume of liquid culture was prepared by adding all sterile stock solution components to 912.5 mL of Milli-Q water in an acid-cleaned HDPE bottle on a balance. *FeSO4 added as 57FeSO4 spike separately after all other components combined. Completed M9 minimal media was 0.02 µm filtered prior to use.	Download
Figure3.PNG (151.65 KB)	Plain Text	Figure 3: Flowchart of the Tracing 57Fe to E. coli phages T4 & T5 Experimental method. First, cell cultures were grown and aliquoted into triplicate samples of each treatment: T4 infected (A, B, C), T5 infected (M, N, O), Bacterial Control (D, E, F), and Blank Control (G, H, I). Cell cultures were rinsed to remove excess 57Fe, then lysed by phage T4 infection, phage T5 infection, or chloroform for the bacterial lysis control. The lysates are then purified for the phage by centrifugation, filtration, sucrose ultracentrifugation, and dialysis.	Download
Figure2.PNG (129.69 KB)	Portable Network Graphics (.png)	Figure 2: Schematic of E. coli cell preparation	Download
Figure1.PNG (34.65 KB)	Portable Network Graphics (.png)	Growth curve for E. coli ZK126 measured on a spectrophotometer. Mid-logarithmic growth (indicated by shaded area) was an OD600= 0.200-0.500.	Download

Related Datasets

No Related Datasets

Related Publications

Methods

Gledhill, M. (2012). The organic complexation of iron in the marine environment: a review. Frontiers in Microbiology, 3. doi:10.3389/fmicb.2012.00069

Methods

Kutter, E., & Sulakvelidze, A. (2004). Bacteriophages: biology and applications. CRC Press.

Methods

Noble, R., & Fuhrman, J. (1998). Use of SYBR Green I for rapid epifluorescence counts of marine viruses and bacteria. Aquatic Microbial Ecology, 14, 113–118. doi:10.3354/ame014113

Dataset: Iron concentrations of phage from experiments of iron-labelled E. coli infected with T4 and T5 bacteriophage, 2018 and 2019.

Principal Investigator: Mya Breitbart (University of South Florida)

Principal Investigator: Kristen Nicolle Buck (University of South Florida)

Co-Principal Investigator: Chelsea Bonnain (University of South Florida)

Co-Principal Investigator: Salvatore Caprara (University of South Florida)

BCO-DMO Data Manager: Nancy Copley (Woods Hole Oceanographic Institution)

Project: EAGER: Iron-Virus Interactions in the Ocean (Fe-Virus)

Abstract

ERDDAP

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Dataset: Iron concentrations of phage from experiments of iron-labelled E. coli infected with T4 and T5 bacteriophage, 2018 and 2019.

Principal Investigator: Mya Breitbart (University of South Florida)

Principal Investigator: Kristen Nicolle Buck (University of South Florida)

Co-Principal Investigator: Chelsea Bonnain (University of South Florida)

Co-Principal Investigator: Salvatore Caprara (University of South Florida)

BCO-DMO Data Manager: Nancy Copley (Woods Hole Oceanographic Institution)

Project: EAGER: Iron-Virus Interactions in the Ocean (Fe-Virus)

Abstract

ERDDAP

Metadata

XXX

XX

X

Related Datasets

Related Publications