Day 1: Transfect cell lines

15 breast cancer cell lines and 3 normal breast cell lines are transfected using Lullaby and custom designed metabolic enzyme library for 1 day under normal and hypoxia conditions.

Day 2: Change the media

Change for fresh culture media and culture the plates for further 3 days under the respective normal and hypoxia condition.

Day 5: Fix the plates with 80% EthOH and stain

Stain with capase-3 antibody to detect the Apotosis and stain with DAPI for nuclear counting.

Readout

Acumen Explorer eX3 laser scanning cytometer was used to determine cell number per well and Caspase-3 intensity.

Screen Status:	Primary
Screen Overview:	Primary Screen
Screener:	Franzi Baenke (Schulze Lab). Extension:2049, Rm 113
Library:	Glucose Metabolism Custom Franzi
Library Description:	Re-arrangement of Glucose Metabolism library (libID 95) with additional siRNAs ordered seperately. 3 plates
Library Supplier:	Dharmacon
Library Format:	3 plate(s) in 96 well format
Replicate Info:	3 replicates
Publications:	Functional screening identifies MCT4 as a key regulator of breast cancer cell metabolism and survival.. Baenke et al., 2015
Keywords:	Breast Cancer, Metabolism, Viability
Cell Line:	ZR-75-1

Screen Method