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DEPARTAMENTO DE CIÊNCIAS DA VIDA ... - Estudo Geral

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36<br />

clone SAM1; mouse Pe-Cy7 anti-human CD13 IgG1, clone WM15; mouse PE antihuman<br />

CD73 IgG1, clone AD2; mouse APC anti-human CD90 IgG1, clone 5E10; mouse<br />

PO anti-human CD45 IgG1, clone HI30; mouse PB anti-human CD11b IgG1, clone<br />

ICRF44; mouse APC-H7 anti-human HLA-DR IgG2a, clone G46-6. The staining and image<br />

acquisition and analyze<br />

II.2.5 - Preparation of polyacrylamide hydrogels<br />

Since polyacrylamide hydrogels were polymerized on top of autoclaved glass coverslips<br />

(15x15 cm or 24x50 cm), a treatment to allow the establishment of chemical covalent<br />

links between the coverslip and the hydrogel using a silane agent was necessary<br />

(adapted from Hoffecker et al., 2011).<br />

A dilution of 3-(Trimethoxysilyl) propyl methacrylate in ethanol of 1:200 was made and<br />

just before use was added 3% of diluted acetic acid (1:10 glacial acetic acid: water).<br />

This solution was placed on top of cleaned coverslips, allowed to react for 3 minutes<br />

and then the reactive coverslips were rinsed with ethanol to remove the residual<br />

reagent and dried (Hoffecker, et al. 2011).<br />

After the glass coverslips treatment with the silane agent, a saturated solution of N-<br />

Acryloxysuccinimide (NHS) was prepared in toluene and kept covered to prevent<br />

toluene evaporation. The NHS solution was used in the hydrogel composition to allow<br />

the functionalization of the hydrogel surface with covalently bound proteins to allow<br />

for cell adherence. Then, the solution of acrylamide, bis-acrylamide, water and TEMED<br />

(Tetramethylethylenediamine) was prepared according to Table I. The solution was<br />

degassed for 30 min (using a Vacuum Aspiration System from INTEGRA Biosciences).<br />

Afterwards, the solutions of NHS and ammonium persulfate (APS) were added to the<br />

hydrogel solutions and briefly mixed (adapted from Cretu, et al 2010).

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