Atomic Force Microscopy of Bacterial Cells

AFM experimentation was conducted as previously(Eskandarian et al., 2017 (link)). In short, polydimethylsiloxane (PDMS) – coated coverslips were prepared by spin-coating a mixture of PDMS at a ratio of 15:1 (elastomer:curing agent) with hexane (Sigma 296090) at a ratio of 1:10 (PDMS:hexane) (Koschwanez et al., 2009 (link); Thangawng et al., 2007 (link)). A 50 µl filtered (0.5 µm pore size PVDF filter – Millipore) aliquot of bacteria grown to mid-exponential phase and concentrated from 2 to 5 ml of culture was deposited onto the hydrophobic surface of a PDMS-coated coverslip and incubated for ~20 min to increase surface interactions between bacteria and the coverslip. 7H9 medium (~3 ml) was supplied to the sample so as to immerse the bacterial sample and the AFM cantilever in fluid. The AFM imaging mode, Peak Force QNM, was used to image bacteria with a Nanoscope five controller (Veeco Metrology) at a scan rate of 0.5 Hz and a maximum Z-range of 12 µm. A ScanAsyst fluid cantilever (Bruker) was used. Height, peak force error, DMT modulus, and log DMT modulus were recorded for all scanned images in the trace and retrace directions. Images were processed using Gwyddion (Department of Nanometrology, Czech Metrology Institute). ImageJ was used for extracting bacterial cell profiles in a tabular form.

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Baranowski C., Welsh M.A., Sham L.T., Eskandarian H.A., Lim H.C., Kieser K.J., Wagner J.C., McKinney J.D., Fantner G.E., Ioerger T.R., Walker S., Bernhardt T.G., Rubin E.J, & Rego E.H. (2018). Maturing Mycobacterium smegmatis peptidoglycan requires non-canonical crosslinks to maintain shape. eLife, 7, e37516.

Publication 2018

ScanAsyst fluid cantilever

Bacterial Elastomer Hexane Polydimethylsiloxane Pvdf

Corresponding Organization :

Other organizations : Harvard University, National University of Singapore, École Polytechnique Fédérale de Lausanne, Texas A&M University, Yale University

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Variable analysis

independent variables

Spin-coating a mixture of PDMS at a ratio of 15:1 (elastomer:curing agent) with hexane (Sigma 296090) at a ratio of 1:10 (PDMS:hexane)

dependent variables

Height
Peak force error
DMT modulus
Log DMT modulus

control variables

Bacteria grown to mid-exponential phase and concentrated from 2 to 5 ml of culture
Deposition of 50 µl filtered (0.5 µm pore size PVDF filter – Millipore) bacterial sample onto the hydrophobic surface of a PDMS-coated coverslip
Incubation of the bacterial sample for ~20 min to increase surface interactions between bacteria and the coverslip
Supply of 7H9 medium (~3 ml) to immerse the bacterial sample and the AFM cantilever in fluid
Use of Peak Force QNM imaging mode with a Nanoscope five controller (Veeco Metrology) at a scan rate of 0.5 Hz and a maximum Z-range of 12 µm
Use of a ScanAsyst fluid cantilever (Bruker)

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