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Supplemental Materials Cytotoxic Effect of Trabectedin In Human Adrenocortical Carcinoma Cell Lines and Primary Cells

Andrea Abate, Elisa Rossini, Sara A. Bonini, Martina Fragni, Deborah Cosentini, Guido A.M. Tiberio, Diego Benetti; Constanze Hantel, Marta Laganà, Salvatore Grisanti, Massimo Terzolo, Maurizio Memo, Alfredo Berruti and Sandra Sigala

1. Evaluation of DNA Fragmentation

NCI-H295R cells were treated with the IC50 value of trabectedin for 4 days. DNA was extracted from cells using Apoptotic DNA Ladder Kit (ThermoFisher, Waltham, USA) and processed according to the manufactured. The DNA was loaded on 1.2% agarose-gel, containing 0.5 µg/mL ethidium bromide. Ethidium bromide-stained DNA was visualized by transillumination with UV light and was photographed.

2. Double staining AO/EtBr

NCI-H295R cells were treated with the IC50 value of trabectedin for 4 days. A double staining with acridine orange (AO) and ethidium bromide (EtBr) was performed to visualize and quantify the number of viable, apoptotic and necrotic cells, as described in [49].

Cells were examined by a Zeiss LSM 510 META confocal laser-scanning microscope (Carl Zeiss AG, Germany). Several fields, randomly chosen, were digitalized and scored by using the NIH Image J software.

Figure S1. Effect of trabectedin on DNA integrity. NCI-H295R cells were treated with trabectedin at its IC50 for 4 days. DNA from treated and untreated cells was extracted and loaded on agarose-gel, containing ethidium bromide.

C

Trab

Figure S2. Trabectedin promoted apoptotic cell death in NCI-H295R cells.NCI-H295R cells were treated for 4 days with trabectedin at its IC50 and then stained with AO/EtBr. (A) Viable (green), apoptotic (yellow) and necrotic (red) cells were scored under a confocal laser-scanning microscope. Bars represent the percentage of each cell colour vs the total number of cell/field. * p < 0.01 vs. untreated apoptotic (yellow) cells. (B) The images were representative of several acquired fields (a) untreated and (b) trabectedin-treated cells. Magnification, 10×.

A

% of viable, apoptotic and necrotic cells/field

untreated

IC50 Trabectedin

100

80

60-

40-

*

20

0

B

a

b

200 pm

200 um

Figure S3. Cytotoxic effect of trabectedin on SW13 cell line. (A) SW13 cells were treated for 3 days with increasing concentrations (0.0625-0.75 nM) of trabectedin. (B) SW13 cells were treated with 0.09 nM trabectedin for 3 days, then trabectedin was withdrawn from medium and cells were kept in culture for further 3 days. Cell viability was analyzed by MTT assay. Results are expressed as percent of viable cells vs untreated cells ±SD ;* p<0.01, *** p<0.0001, *** p < 0.0001 vs trabectedin-treated cells; # p < 0.01 vs trabectedin-treated cells.

Cell viability (% vs CTRL)

100

*

80-

60-

40-

20-

0

-10.5

-10.0

-9.5

-9.0

Trabectedin [LogM]

A

Survival vs control [%]

8 8 8 8 8

withdrawn 3 days

0

Trabectedin

-

+

+

B

B-catenin and GAPDH

M.W.

1

2

[KDa]

115

80

58

50

31

1: Ctrl

2: IC50

Lane nºB-catenin intenityGAPDH intensityB-catenin/ GAPDHRatio
10.19250.26400.7292100
20.25700.35300.728099.83

Nucleolin and GAPDH

M.W. [KDa]

Nucleolin and B-catenin 1 2 3 4

1 2 3 4

115

80

58

50

31

1: Ctrl EC (Cytosolic Extract)

2: Ctrl EN (Nuclear Extract)

3: IC50 EC

4: IC50 EN

Lane nºB-catenin intensityNucleolin intensityB-catenin/ nucleolinRatio
20.07700.13500.5704100
40.05600.19250.290951

Figure S4. Whole western blots of Figure 4.

Figure S5. Representative figure of subfractions proteins of NCI-H295R. EN = Nuclear Extract, EC = Cytosolic Extract.

EN EC EN EC

110kDa

nucleolin

37kDa

GAPDH

Figure S6. Trabectedin exposure affects the subcellular localization of ß-catenin in NCIH295R cells. Cells were treated with 0.15 nM trabectedin for 2, 3 and 4 days. After 4 days of treatment, trabectedin was withdrawn from medium and cells were kept in culture for further 2 days. Untreated and trabectedin treated cells were analyzed for ß-catenin localization following by incubation with Hoechst for nuclear staining. For each panel, the top-left insert: Hoechst; top-right insert; ß-catenin; bottom-left insert: constitutive proteasome subunit PSMB5; bottom-right insert: merge. The scale bar of 50 um is automatically inserted by the software ZEN Black.

Ctrl

IC50

2 days

50 pm

50 μm

50 pm

50 um

50 μm

50 μm

50 pm

50 μm

3 days

50 μm

50 pm

50 pm

50 μm

50 um

50 um

50 μm

50 μm

2 days withdrawn

50 μm

50 μm

50 μm

50 mm

50 μm

50 pm

50 μm

50 μm

CC

7

BY

@ 2020 by the authors. Licensee MDPI, Basel, Switzerland. This article is an open access article distributed under the terms and conditions of the Creative Commons Attribution (CC BY) license (http://creativecommons.org/licenses/by/4.0/).

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