GSM8329974: Cas12a-SLCxSLC_sublib2_input_rep2; synthetic construct; O... - SRA

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SRX24932934: GSM8329974: Cas12a-SLCxSLC_sublib2_input_rep2; synthetic construct; OTHER
2 ILLUMINA (Illumina NovaSeq 6000) runs: 353.3M spots, 35.7G bases, 12.7Gb downloads

External Id: GSM8329974_r1

Submitted by: CeMM Research Center for Molecular Medicine of the Austrian Academy of Sciences

Study: Mapping genetic interactions in the SLC Transporter Superfamily.

PRJNA1124096 • SRP514040 • All experiments • All runs

show Abstracthide Abstract

Transporters mediate and control the flux of molecules across compartmental membranes. The human genome encodes 1500 genes with transport functions, of which the solute carriers (SLCs) form the largest superfamily with more than 450 members. Over 250 different SLCs are expressed in a typical human cell, many exhibiting overlapping expression patterns and substrate specificities. The collective role of these often seemingly redundant transporters in defining cellular outcomes, such as cell survival, remains unclear. Here, we performed pooled combinatorial KO screens to identify genetic interactions between 258 expressed SLCs, and between a subset of SLCs and selected metabolic enzymes under different growth conditions using both CRISPR-Cas12a and -Cas9 double knockout systems in the colorectal carcinoma cell line HCT116. Overall design: Pooled combinatorial KO screens with proliferation read out.

Sample: Cas12a-SLCxSLC_sublib2_input_rep2

SAMN41842984 • SRS21637329 • All experiments • All runs

Organism: synthetic construct

Library:

Name: GSM8329974

Instrument: Illumina NovaSeq 6000

Strategy: OTHER

Source: OTHER

Selection: other

Layout: SINGLE

Construction protocol: For the Cas12a-Metal-SLCxSLC, Cas12a- and Cas9-SLCxEnzymes, and Cas12a- and Cas9-SLCxSLC, gDNA was purified from 2x10e7 (QIAamp DNA Mini Kit), 1.7x10e7 (QIAGEN Genomic-tip 100/G) or 2.2x10e8 cells (QIAGEN Genomic-tip 500/G), respectively. gDNA from Cas12a- and Cas9-SLCxSLC screens was digested with restriction enzymes to improve PCR amplification of sgRNA regions. Up to 1.5 mg gDNA was digested with 200 U PacI (Cas12a-SLCxSLC) or 100 U PacI and 100 U XbaI (Cas9-SLCxSLC) (all NEB) for 48 hours. sgRNA sequences from Cas12a library gDNA samples were amplified with barcoded FW and RV primer that introduce Illumina adapter and read1 sequencing primer binding sites. Up to 1.2 mg gDNA was used as template in 12 ml volume (divided in 96 x 125 µl PCRs) in the following program: 98°C for 30 sec.; 5 cycles: 98°C for 10 sec., 61°C for 30 sec, 72°C for 30 sec; 19 cycles: 98°C for 10 sec., 72°C for 1 min.; 72°C for 2 min. For the samples of the metal transporter and SLC family-wide sub-screen 1, Q5 Polymerase (NEB) was used, SLC vs SLC sub-screen 2-4 and SLC vs metabolic enzymes samples were processed with self-purified Pfu-Sso7d polymerase and Phusion HF buffer (NEB). Primer sequences are shown in Supplementary Table SX. PCR products we double size selected with DNA purification bads and multiplexed for Illumina sequencing. sgRNA sequences from Cas9 library gDNA samples were first amplified with staggered FW and RV primer that contain partial Illumina adapter sequences at the 5' end using the same PCR program as above. Up to 1.2 mg gDNA was used as template (125 µg/125 µl volume PCR) and amplified with self-purified Pfu-Sso7d polymerase. An aliquot of the pooled amplified PCR products was double size selected with DNA purification bads and purified fragments were barcoded in a second PCRs (98°C for 30 sec; 6-8 cycles: 98°C for 10 sec., 61°C for 30 sec, 72°C for 30 sec; 72°C for 2 min). PCR products we double size selected with DNA purification bads and multiplexed for Illumina sequencing.

Runs: 2 runs, 353.3M spots, 35.7G bases, 12.7Gb

Run	# of Spots	# of Bases	Size	Published
SRR29419728	176,670,526	17.8G	6.3Gb	2024-06-19
SRR29419729	176,595,307	17.8G	6.3Gb	2024-06-19

ID:: 33269177

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