A simple, inexpensive method for preparing cell lysates suitable for downstream reverse transcription quantitative PCR

Shatzkes, Kenneth; Teferedegne, Belete; Murata, Haruhiko

doi:10.1038/srep04659

Cited by 58 publications

(69 citation statements)

References 17 publications

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“…Generally, it has been shown that miRNAs are highly stable in cell lysates and can be stored at −20 and/or −80°C for days. 18,19 In our proof-ofconcept test of freeze−thaw cell lysate, the endogenous miR-21 signal was decreased by ∼50% compared to fresh cell lysates ( Figure S4). This signal decrease is probably due to freeze/ thaw temperatures (here, −20°C/room temperature) or absence of RNase inhibitor; a previous study demonstrated that RNA stability was enhanced when stored at −80°C or thawed at 4°C or RNase inhibitor added.…”

Section: ■ Experimental Sectionmentioning

confidence: 99%

“…Previously, Ho et al has reported microRNA LODs of 200 cells, 19 which is within an order of magnitude of the LOD obtained with our hydrogel-based detection. Even though some recent studies on direct miRNA measurements demonstrate high sensitivity (1−1000 cells), 18,20 their measurements are based on target-based amplification of qRT-PCR. This targetbased amplification often introduces sequence bias.…”

Section: ■ Experimental Sectionmentioning

confidence: 99%

“…This signal decrease is probably due to freeze/ thaw temperatures (here, −20°C/room temperature) or absence of RNase inhibitor; a previous study demonstrated that RNA stability was enhanced when stored at −80°C or thawed at 4°C or RNase inhibitor added. 18 For better assay reliability and sensitivity, it is possible to further optimize our assay protocol in the future.…”

Section: ■ Experimental Sectionmentioning

confidence: 99%

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Encoded Hydrogel Microparticles for Sensitive and Multiplex microRNA Detection Directly from Raw Cell Lysates

et al. 2016

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In recent years, microRNAs (miRNAs) have emerged as promising diagnostic markers because of their unique dysregulation patterns under various disease conditions and high stability in biological fluids. However, current methods of analyzing miRNA levels typically require RNA isolation, which is cumbersome and time-consuming. To achieve high-throughput and accurate miRNA profiling, this study eliminates the need for purification steps by detecting miRNA directly from raw cellular lysate using nonfouling polyethylene glycol microparticles. In contrast to recent studies on direct miRNA measurements from cell lysate, our hydrogel-based system provides high-confidence quantification with robust performance. The lysis buffer for the assay was optimized to maximize reaction and labeling efficiency, and this assay has a low limit of detection (<1000 cells) without target amplification. Additionally, the capability for multiplexing was demonstrated through analyzing the levels of three endogenous miRNAs in 3T3 cell lysate. This versatile platform holds great potential for rapid and reliable direct miRNA quantification in complex media, and can be further extended to single-cell analysis by exploiting the flexibility and scalability of our system.

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Section: ■ Experimental Sectionmentioning

confidence: 99%

Section: ■ Experimental Sectionmentioning

confidence: 99%

Section: ■ Experimental Sectionmentioning

confidence: 99%

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Encoded Hydrogel Microparticles for Sensitive and Multiplex microRNA Detection Directly from Raw Cell Lysates

et al. 2016

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“…Cells were washed with cold PBS once and lysed in the Real-time cell lysis buffer containing 10mM Tris pH 7.4, 0.25% Igepal CA-630, and 150mM NaCl for 5 mins [18]. Cell lysates were directly used for real-time as the amplification templates.…”

Section: Real-time Quantitative Pcr (Rt-qpcr)mentioning

confidence: 99%

Histone Acetyltransferase (HAT) P300/CBP Inhibitors Induce Synthetic Lethality in PTEN-Deficient Colorectal Cancer Cells through Destabilizing AKT

Liu¹,

Yang²,

Shi³

et al. 2020

Int. J. Biol. Sci.

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PTEN, a tumor suppressor, is found loss of function in many cancers, including colorectal cancer. To identify the synthetic lethal compounds working with PTEN deficiency, we performed a synthetic lethality drug screening with PTEN-isogenic colorectal cancer cells. From the screening, we found that PTEN -/colorectal cancer cells were sensitive to anacardic acid, a p300/CBP histone acetyltransferase (HAT) inhibitor. Anacardic acid significantly reduced the viability of PTEN -/-cells not in PTEN +/+ cells via inducing apoptosis. Inhibition of HAT activity of p300/CBP by anacardic acid reduced the acetylation of histones at the promoter region and inhibited the transcription of Hsp70 family of proteins. The down-regulation of Hsp70 family proteins led to the reduction of AKT-Hsp70 complex formation, AKT destabilization and decreased the level of phosphorylated AKT at Ser473, all of which are vital for the survival of PTEN -/colorectal cells. The synthetic lethality effect of anacardic acid was further validated in tumor xenograft mice models, where PTEN -/-colorectal tumors showed greater sensitivity to anacardic acid treatment than PTEN +/+ tumors. These data suggest that anacardic acid induced synthetic lethality by inhibiting HAT activity of p300/CBP, thereby reducing Hsp70 transcription and destabilizing AKT in PTEN deficient colorectal cancer cells.

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“…Cell lysate was then prepared by aspirating the culture media using the GNF Systems (San Diego, CA) WDII plate washer, and then the cells were washed with 100 μL of cold PBS, removing as much of the wash solution from each well as possible. The cells were then lysed by the addition of 15 μL of lysis buffer (10 mM Tris-HCl, pH 7.4, 0.25% IGEPAL, 150 mM NaCl, final concentrations, dissolved using DNase/ RNase-free water, all from Sigma) as described by Shatzkes et al 20 The cells were lysed by incubation for 30 min at room temperature. During this time, the PCR master mix (Roche Diagnostics, Indianapolis, IN) was prepared, including Taqman primers for actin and CYR61, and then 900 nL of the master mix was dispensed to the Roche LightCycler 1536 well assay plate using the Thermo Combi nL.…”

Section: Qpcr To Measure Cyr61 Gene Expressionmentioning

confidence: 99%

Activation of Yap-Directed Transcription by Knockdown of Conserved Cellular Functions

et al. 2016

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The Yap-Hippo pathway has a significant role in regulating cell proliferation and growth, thus controlling organ size and regeneration. The Hippo pathway regulates two highly conserved, transcription coactivators, YAP and TAZ. The upstream regulators of the Yap-Hippo pathway have not been fully characterized. The aim of this study was to use a siRNA screen, in a liver biliary cell line, to identify regulators of the Yap-Hippo pathway that allow activation of the YAP transcription coactivator at high cell density. Activation of the YAP transcription coactivator was monitored using a high-content, image-based assay that measured the intracellular localization of native YAP protein. Active siRNAs were identified and further validated by quantification of CYR61 mRNA levels (a known YAP target gene). The effect of compounds targeting the putative gene targets identified as hits was also used for further validation. A number of validated hits reveal basic aspects of Yap-Hippo biology, such as components of the nuclear pore, by which YAP cytoplasmic-nuclear shuttling occurs, or how proteasomal degradation regulates intracellular YAP concentrations, which then alter YAP localization and transcription. Such results highlight how targeting conserved cellular functions can lead to validated activity in phenotypic assays.

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A simple, inexpensive method for preparing cell lysates suitable for downstream reverse transcription quantitative PCR

Cited by 58 publications

References 17 publications

Encoded Hydrogel Microparticles for Sensitive and Multiplex microRNA Detection Directly from Raw Cell Lysates

Encoded Hydrogel Microparticles for Sensitive and Multiplex microRNA Detection Directly from Raw Cell Lysates

Histone Acetyltransferase (HAT) P300/CBP Inhibitors Induce Synthetic Lethality in PTEN-Deficient Colorectal Cancer Cells through Destabilizing AKT

Activation of Yap-Directed Transcription by Knockdown of Conserved Cellular Functions

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