Internalization of AuNP-Capped MSN in A549 Cells

A549 cells were cultured 48 h before imaging with cell culture medium, using our previously published methods.^{22 (link)} Next the culturing medium was removed and cells were washed with 1× PBS. Twenty-four h prior to incubation with AuNP-capped MSN, cells were placed in a cell culture medium containing 500 µM α-lipoic acid (Sigma-Aldrich).^{23 (link)} Cells were kept in the α-lipoic acid culturing medium for 24 h, and then the AuNP-capped MSN were added. 200 µL of nanoparticles were added to the Petri dish with 1 mL of new culturing medium. Cells were incubated for 2 h to naturally internalize the AuNP-capped MSN.^{24 (link)} After incubation, the culturing medium and nanoparticle solution were removed, and the cells were washed again with 1× PBS. After the cells were washed with PBS, a slide was prepared for imaging. Two pieces of double sided tape were placed across the slide parallel to one another. Between the two pieces of tape some culturing medium was pipetted, and the glass coverslip was secured on the glass slide with the tape. During imaging, the cell sample was scanned vertically with a computer controlled vertical stage scanner (Sigma Koki, model no. SGSP-60YAM) attached to the fine-tune knob of the microscope. A 540 nm (10 nm fwhm) bandpass filter was used to image the cells; the sample was vertically scanned every 10 min for 3 h.

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Augspurger A.E., Sun X., Trewyn B.G., Fang N, & Stender A.S. (2018). Monitoring the Stimulated Uncapping Process of Gold-Capped Mesoporous Silica Nanoparticles. Analytical chemistry, 90(5), 3183-3188.

Publication 2018

α-lipoic acid

A549 cells Cell culture Cells Dish Microscope Placed cell α lipoic acid

Corresponding Organization : Ohio University

Other organizations : Colorado School of Mines

Top 5 similar protocols

Variable analysis

independent variables

Incubation with AuNP-capped MSN

dependent variables

Internalization of AuNP-capped MSN by cells
Imaging of cells over a 3-hour period

control variables

A549 cell line
Cell culture medium
Incubation time with AuNP-capped MSN (2 hours)
Vertical scanning of cell sample every 10 minutes for 3 hours
Use of 540 nm (10 nm fwhm) bandpass filter

positive controls

None specified

negative controls

None specified

Annotations

Based on most similar protocols

The cultures should be maintained at 37 °C in a humidified atmosphere with 5% CO2 as specified in Protocol 1.

Replicated wells containing the cells and cell-culture medium only (no AuNPs) should be prepared as the negative control, as mentioned in Protocol 1.

After 3 h incubation with AuNPs, the cells should be washed three times with PBS to remove extra nanoparticles, as described in Protocol 1.

For imaging, the cell sample should be scanned vertically with a computer-controlled vertical stage scanner, as mentioned in the Input protocol.

A 540 nm (10 nm fwhm) bandpass filter should be used to image the cells, as specified in the Input protocol.

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