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        <gco:CharacterString>Lagrangian Structure and Stretching in Bacterial Turbulence Dataset Description: &amp;lt;p&amp;gt;&amp;lt;strong&amp;gt;Velocity Field Variables:&amp;lt;/strong&amp;gt;&amp;lt;/p&amp;gt;

&amp;lt;p&amp;gt;&amp;lt;em&amp;gt;U:&amp;lt;/em&amp;gt;&amp;amp;nbsp;u-component of the velocity fields&amp;lt;/p&amp;gt;

&amp;lt;p&amp;gt;&amp;lt;em&amp;gt;V:&amp;lt;/em&amp;gt;&amp;amp;nbsp;v-component of the velocity fields&amp;lt;/p&amp;gt;

&amp;lt;p&amp;gt;&amp;lt;em&amp;gt;X,Y&amp;lt;/em&amp;gt;: XY coordinates produced from the PIV analysis (meshgrid layout)&amp;lt;/p&amp;gt;

&amp;lt;p&amp;gt;&amp;amp;nbsp;&amp;lt;/p&amp;gt;

&amp;lt;p&amp;gt;&amp;lt;strong&amp;gt;Stretching Field Variables:&amp;lt;/strong&amp;gt;&amp;lt;/p&amp;gt;

&amp;lt;p&amp;gt;&amp;lt;em&amp;gt;TINT:&amp;amp;nbsp;&amp;lt;/em&amp;gt;Integration time for tracer particles (s)&amp;lt;/p&amp;gt;

&amp;lt;p&amp;gt;&amp;lt;em&amp;gt;choice:&amp;lt;/em&amp;gt;&amp;amp;nbsp;parameter choices for numerical experiment, see code for details&amp;lt;/p&amp;gt;

&amp;lt;p&amp;gt;&amp;lt;em&amp;gt;stretch:&amp;lt;/em&amp;gt;&amp;amp;nbsp;a Nx1 cell of the stretching field for this particular integration time, where each cell is a frame&amp;lt;/p&amp;gt;

&amp;lt;p&amp;gt;&amp;lt;em&amp;gt;tintegrate:&amp;lt;/em&amp;gt;&amp;amp;nbsp;time vector of the tracer particle integration&amp;lt;/p&amp;gt;

&amp;lt;p&amp;gt;&amp;lt;em&amp;gt;x_field, y_field:&amp;amp;nbsp;&amp;lt;/em&amp;gt;Initial xy coordinates of tracer particle grids. Formed using meshgrid&amp;lt;/p&amp;gt; Methods and Sampling: &amp;lt;p&amp;gt;&amp;lt;strong&amp;gt;Culturing:&amp;lt;/strong&amp;gt;&amp;lt;/p&amp;gt;

&amp;lt;p&amp;gt;Wild-type&amp;amp;nbsp;Bacillus subtilis&amp;amp;nbsp;bacteria (strain OI1084) were taken from −80°C frozen stock and streaked onto 1.5% agar plates prepared with Terrific Broth (TB, Sigma). Plates were incubated at 25°C for 24 hours, after which time a single colony from the plate was used to inoculate an overnight liquid TB culture at 30°C with shaking (200 rpm). The bacterial suspension was then subcultured (1.5 ml of cell culture into 60 ml of pre-warmed TB) and grown at 35°C and 200 rpm for 6 hours to mid-log phase (OD600&amp;amp;nbsp;≈ 0.2). Immediately prior to experiments, dense cell suspensions (∼ 1010&amp;amp;nbsp;cells.ml−1) were prepared by centrifugation at 5000 g for 5 minutes, and the pellet was resuspended with 2&amp;amp;nbsp;μl of fresh TB media.&amp;lt;/p&amp;gt;

&amp;lt;p&amp;gt;&amp;amp;nbsp;&amp;lt;/p&amp;gt;

&amp;lt;p&amp;gt;&amp;lt;strong&amp;gt;Microfluidics and image analysis&amp;lt;/strong&amp;gt;&amp;lt;/p&amp;gt;

&amp;lt;p&amp;gt;Polydimethlysiloxane (PDMS) microfluidic channels were fabricated through soft lithography&amp;amp;nbsp;and plasma bonded to No. 1 thickness glass coverslips. The PDMS channels were thinly cast to ensure ample diffusion of oxygen to the bacterial suspension and prolonged cell activity. Dense cell suspensions were gently loaded into the microfluidic devices via pipette, and the channel inlet and outlet were sealed with wax to prevent residual flows. For all experiments, bacterial suspensions were imaged with brightfield illumination on an inverted microscope (Nikon Ti-E) using a sCMOS camera (Zyla 5.5, Andor Technology) at 40x magnification. Time-resolved velocity fields,&amp;amp;nbsp;u(x,&amp;amp;nbsp;t), of the bacterial suspensions were measured by performing Particle Image Velocimetry (PIV) using PIVLab&amp;amp;nbsp;implemented in MATLAB. The subsequent velocity fields were then lightly smoothed using a Guassian kernel with a standard deviation of one PIV pixel in space and one frame in time.&amp;amp;nbsp;&amp;lt;/p&amp;gt;</gco:CharacterString>
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        <gmx:Anchor xlink:href="http://lod.bco-dmo.org/id/award/783784.rdf" xlink:title="OCE-1829827" xlink:actuate="onRequest">Funding provided by NSF Division of Ocean Sciences (NSF OCE) Award Number: OCE-1829827 Award URL: https://www.nsf.gov/awardsearch/show-award?AWD_ID=1829827</gmx:Anchor>
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        <gmi:MI_Instrument>
          <gmi:identifier>
            <gmd:MD_Identifier>
              <gmd:code>
                <gmx:Anchor xlink:href="http://lod.bco-dmo.org/id/instrument/520.rdf" xlink:title="Camera" xlink:actuate="onRequest">sCOMOS camera (Zyla 5.5, Andor Technology)</gmx:Anchor>
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            <gco:CharacterString>sCOMOS camera (Zyla 5.5, Andor Technology)</gco:CharacterString>
          </gmi:type>
          <gmi:description>
            <gco:CharacterString>PI Supplied Instrument Name: sCOMOS camera (Zyla 5.5, Andor Technology) PI Supplied Instrument Description:For all experiments, bacterial suspensions were imaged with brightfield illumination on an inverted microscope (Nikon Ti-E) using a sCMOS camera (Zyla 5.5, Andor Technology) at 40x magnification. Instrument Name: Camera Instrument Short Name:camera   Instrument Description: All types of photographic equipment including stills, video, film and digital systems. Community Standard Description: http://vocab.nerc.ac.uk/collection/L05/current/311/</gco:CharacterString>
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      <gmi:instrument>
        <gmi:MI_Instrument>
          <gmi:identifier>
            <gmd:MD_Identifier>
              <gmd:code>
                <gmx:Anchor xlink:href="http://lod.bco-dmo.org/id/instrument/675.rdf" xlink:title="Inverted Microscope" xlink:actuate="onRequest">Nikon Ti-E Inverted microscope</gmx:Anchor>
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          <gmi:type>
            <gco:CharacterString>Nikon Ti-E Inverted microscope</gco:CharacterString>
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            <gco:CharacterString>PI Supplied Instrument Name: Nikon Ti-E Inverted microscope PI Supplied Instrument Description:For all experiments, bacterial suspensions were imaged with brightfield illumination on an inverted microscope (Nikon Ti-E) using a sCMOS camera (Zyla 5.5, Andor Technology) at 40x magnification. Instrument Name: Inverted Microscope Instrument Short Name:   Instrument Description: An inverted microscope is a microscope with its light source and condenser on the top, above the stage pointing down, while the objectives and turret are below the stage pointing up. It was invented in 1850 by J. Lawrence Smith, a faculty member of Tulane University (then named the Medical College of Louisiana).

Inverted microscopes are useful for observing living cells or organisms at the bottom of a large container (e.g. a tissue culture flask) under more natural conditions than on a glass slide, as is the case with a conventional microscope. Inverted microscopes are also used in micromanipulation applications where space above the specimen is required for manipulator mechanisms and the microtools they hold, and in metallurgical applications where polished samples can be placed on top of the stage and viewed from underneath using reflecting objectives.

The stage on an inverted microscope is usually fixed, and focus is adjusted by moving the objective lens along a vertical axis to bring it closer to or further from the specimen. The focus mechanism typically has a dual concentric knob for coarse and fine adjustment. Depending on the size of the microscope, four to six objective lenses of different magnifications may be fitted to a rotating turret known as a nosepiece. These microscopes may also be fitted with accessories for fitting still and video cameras, fluorescence illumination, confocal scanning and many other applications. Community Standard Description: http://vocab.nerc.ac.uk/collection/L05/current/LAB05/</gco:CharacterString>
          </gmi:description>
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