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3051 - 3100 of 4002 citations for Hexadecanoic acid reaction products with tetraethylenepentamine since 2020

• Tautomerization constrains the accuracy of codon-anticodon decoding

  Andriy Kazantsev, Zoya Ignatova, bioRxiv - Biophysics 2020

  Quote: ... we first optimized the wb-WC reaction path in G○U in gas phase using nudged elastic band (NEB) method at B3LYP-D3BJ/def2-TZVP level (Fig ...
• Cockayne Syndrome B protein selectively interacts and resolves intermolecular DNA G-quadruplex structures

  Denise Liano, Marco Di Antonio, bioRxiv - Biochemistry 2021

  Quote: ... The reactions were stopped by addition of 2 μl of no SDS-purple gel loading dye (New England BioLabs) or 50% glycerol ...
• Cell-Free Characterization of Coherent Feed-Forward Loop-Based Synthetic Genetic Circuits

  Pascal A. Pieters, et al., bioRxiv - Synthetic Biology 2021

  Quote: Linear DNA templates for expression in IVTT reactions were created by PCR using Phusion High-Fidelity DNA Polymerase (NEB) with primers pBEST_LinL_F and pBEST_LinL_R (Table S1 ...
• Transcription and splicing dynamics during early Drosophila development

  Pedro Prudêncio, et al., bioRxiv - Molecular Biology 2021

  Quote: ... washed with 100 μl of 1x MNase Buffer and incubated in 100μl of MNase reaction mix (1x MNase buffer and 30 gel unit/μl MNase (New England Biolabs)) during 3 min at 37°C with mix at 1400rpm ...
• An expanded toolkit for Drosophila gene tagging using synthesized homology donor constructs for CRISPR mediated homologous recombination

  Oguz Kanca, et al., bioRxiv - Genetics 2021

  Quote: ... The Golden Gate Assembly reaction was set in 200µl PCR tubes (ThermoScientific AB2000) with 2.5 µl 10X T4 DNA ligase buffer (NEB B0202S), 0.5 µl T4 DNA ligase (NEB M0202L) ...
• NASP maintains histone H3–H4 homeostasis through two distinct H3 binding modes

  Hongyu Bao, et al., bioRxiv - Biochemistry 2021

  Quote: ... 2 μl of this lysate was directly used for PCR reactions with 2× Taq start master mix (M0496L, NEB), and the two NASP clone screening primers (see primer table) ...
• Freeze-thaw Cycles Enable a Prebiotically Plausible and Continuous Pathway from Nucleotide Activation to Nonenzymatic RNA Copying

  Stephanie J. Zhang, et al., bioRxiv - Biochemistry 2021

  Quote: ... 0.1 μg cDNA was added to a 50 μl Q5 Hot Start High-Fidelity DNA Polymerase PCR reaction with 0.2 μM each of NEBNext SR Primer for Illumina and NEBNext Index Primer for Illumina (NEB) and run for 6 cycles with a 15 s 62 °C extension step ...
• Targeted regulation of episomal plasmid DNA expression in eukaryotic cells with a methylated-DNA-binding activator

  Isioma Enwerem-Lackland, et al., bioRxiv - Synthetic Biology 2021

  Quote: Sub-parts (modules, Supplemental Table 1) were amplified via high-fidelity polymerase chain reaction (PCR) (New England Biolabs #M0491S) using dsDNA templates and ssDNA primers listed in Supplemental Table 2 ...
• Linking plasmid-based beta-lactamases to their bacterial hosts using single-cell fusion PCR

  Peter J. Diebold, et al., bioRxiv - Microbiology 2021

  Quote: ... 20 μl qPCR reactions were prepared in duplicate as follows: 1x Luna Universal Probe qPCR Master Mix (NEB M3004L), 300 nM of forward and reverse primer ...
• Production of human translation-competent lysates using dual centrifugation

  Lukas-Adrian Gurzeler, et al., bioRxiv - Molecular Biology 2021

  Quote: ... sequence in a reaction containing 40 ng/μl DNA (4 μg total) and 0.5 U/μl restriction enzyme (HindIII-HF; NEB, Cat ...
• Chlamydia trachomatis Encodes a Dynamic, Ring-Forming Bactofilin Critical for Maintaining Cell Size and Shape

  Mary R. Brockett, et al., bioRxiv - Microbiology 2020

  Quote: ... The products of the HiFi reaction were transformed into either NEB10β (for chlamydial transformation plasmids) or NEB5αIq (for BACTH) competent cells (NEB) and plated on appropriate antibiotics ...
• Potential universal PCR method to detect decapod hepanhamaparvovirus (DHPV) in crustaceans

  Jiraporn Srisala, et al., bioRxiv - Molecular Biology 2020

  Quote: ... the first step PCR reaction was performed in a 12.5 μl mixture containing 1X OneTaq Hot Start Master Mix (NEB), 0.4 μM of each DHPV-U 1538F and DHPV-U 1887R primer and 20 ng of DNA template ...
• Proteogenomic single cell analysis of skeletal muscle myocytes

  Katherine M. Fomchenko, et al., bioRxiv - Genomics 2020

  Quote: ... Capture plate wells contained 5 µl of capture solution (1:500 Phusion High-Fidelity Reaction Buffer, New England Biolabs; 1:250 RnaseOUT Ribonuclease Inhibitor ...
• Unbiased profiling of CRISPR RNA-guided transposition products by long-read sequencing

  Phuc Leo H. Vo, et al., bioRxiv - Molecular Biology 2021

  Quote: ... the resulting supernatant was diluted 20-fold and used as template either for a 12.5 uL PCR reaction with Q5 Polymerase (NEB), or for a 10 uL qPCR reaction with the SsoAdvanced Universal SYBR Green 2X Supermix (BioRad) ...
• CK2 phosphorylation of human papillomavirus 16 E2 on serine 23 promotes interaction with TopBP1 and is critical for E2 plasmid retention function

  Apurva T. Prabhakar, et al., bioRxiv - Molecular Biology 2021

  Quote: ... the beads were incubated with 1 µl CK2 enzyme and 1X CK2 reaction buffer (NEB Inc; catalog no. P6010S) supplemented with 200 µM ATP and 30 mM MgCl2 and rotated for 1 h at 30ºC ...
• Involvement of the Pseudomonas aeruginosa MexAB-OprM efflux pump in the secretion of the metallophore pseudopaline

  Nicolas Oswaldo Gomez, et al., bioRxiv - Microbiology 2020

  Quote: ... PCR reactions for cloning were performed by using Q5® High-Fidelity DNA Polymerase (New England Biolabs, Inc (NEB). All the products sequenced to verify the absence of any mutations (GATC-biotech).
• TReSR: A PCR-compatible DNA sequence design method for engineering proteins containing tandem repeats

  James A Davey, Natalie K Goto, bioRxiv - Synthetic Biology 2023

  Quote: ... Vector DNA was dephosphorylated using quick cow intestinal phosphatase (QCIP) and ligation reactions conducted using T7 DNA ligase (NEB). Purification of DNA products was done by PCR cleanup (E.Z.N.A Cycle Pure Kit ...
• Laboratory evolution of Mycobacterium smegmatis in the presence of a fluoroquinolone leads to extreme drug resistance phenotype through the over-expression of Msmeg_5659-61 efflux pump.

  Deepika Rai, et al., bioRxiv - Systems Biology 2022

  Quote: ... Restriction digestion was done using specific restriction enzymes BamHI and Hind III (0.5 U final concentration) and 1x cut smart reaction buffer (NEB) incubated in the water bath at 37 °C for 2 hours and 15 minutes respectively followed by heat inactivation for 15-20 minutes ...
• Simultaneous inhibition of DNA-PK and Polϴ improves integration efficiency and precision of genome editing

  Sandra Wimberger, et al., bioRxiv - Molecular Biology 2022

  Quote: ... Amplicons for long-range sequencing were generated with Q5 High-Fidelity polymerase in 100 uL reactions (New England Biolabs) including500 nM primers and up to 1000 ng genomic DNA using the following PCR protocol ...
• Dominant Role of Stochastic Processes in Soil Fungal Communities in Pioneer Forests at a Regional Scale

  Xiaowu Man, et al., bioRxiv - Microbiology 2023

  Quote: ... The 30 μl PCR reaction system contained 15 μl of Phusion high-fidelity PCR Master Mix (New England Biolabs), 0.2 μM forward and reverse primers ...
• CRISPR-based editing of the ω- and γ-gliadin gene clusters reduces wheat immunoreactivity without affecting grain protein quality

  Zitong Yu, et al., bioRxiv - Genetics 2023

  Quote: ... The PCR reaction was performed using NEBNext® High-Fidelity 2× PCR Master Mix (New England BioLabs, catalog #M0541) with a reaction volume of 10 ul including 5 ul 2× PCR Master Mix ...
• CRISPR-based engineering of RNA viruses

  Artem Nemudryi, et al., bioRxiv - Molecular Biology 2023

  Quote: ... in a 10 μL reaction in buffer (50 mM Tris-HCl pH 7.5, 1 mM DTT, 1 U/μL RNase Inhibitor (NEB)) and incubated for 1 hour at 37°C ...
• Identification of the alternative sigma factor regulons of Chlamydia trachomatis using multiplexed CRISPR interference

  Nathan D. Hatch, Scot P. Ouellette, bioRxiv - Microbiology 2023

  Quote: ... alkaline phosphatase-treated pBOMBL12CRia(e.v.)::L2 for use in a HiFi reaction according to the manufacturer’s instructions (New England Biolabs (NEB); Cambridge ...
• A Flexible Transgene Integration ‘Landing-Pad’ Toolkit in Human Induced Pluripotent Stem Cells Enables Facile Cellular Engineering, Gene Zygosity Control, and Parallel Transgene Integration

  Aaron H. Rosenstein, et al., bioRxiv - Synthetic Biology 2023

  Quote: ... Reactions were purified according to the ssDNA cleanup protocol from the Monarch PCR cleanup kit (New England Biolabs; T1030L).
• TRPS1 modulates chromatin accessibility to regulate estrogen receptor (ER) binding and ER target gene expression in luminal breast cancer cells

  Thomas G. Scott, et al., bioRxiv - Genomics 2023

  Quote: ... Libraries were amplified by PCR for a total of 8 cycles in 100µL reactions with Phusion polymerase (New England Biolabs). No PAGE purification was performed to ensure that our libraries were not biased against short nascent RNA insertions.
• Differential expression of miRNAs between Young-Onset and Late-Onset Indian colorectal carcinoma patients

  Sumaiya Moiz, et al., bioRxiv - Cancer Biology 2023

  Quote: ... PCR amplification was done in a 25µl reaction with 1 unit of NEB Taq DNA polymerase (NEB Catalog# M0273S), 1x Standard Taq Buffer ...
• Multi-omic study of genome-edited human colonoid models of colorectal cancer reveal genotype-specific patterns of microRNA regulation

  Jonathan W. Villanueva, et al., bioRxiv - Cancer Biology 2023

  Quote: ... Supernatant was removed and chromatin pellets were resuspended in 40 µL 1X DNase I reaction buffer (NEB, Ipswich, MA) containing 1 mM DTT ...
• Differential laboratory passaging of SARS-CoV-2 viral stocks impacts the in vitro assessment of neutralizing antibodies

  Aram Avila-Herrera, et al., bioRxiv - Molecular Biology 2023

  Quote: ... The cDNA was amplified in a 25 µl PCR reactions using 6 µl cDNA and 2X Master mix (NEB). The PCR cycling program was 98 °C for 30 seconds ...
• Nucleolar detention of NONO shields DNA double-strand breaks from aberrant transcripts

  Barbara Trifault, et al., bioRxiv - Molecular Biology 2023

  Quote: ... 37°C with rotation) in 100 µL MNase reaction mix (87 µL ddH2O, 10 µL 10x MNase buffer, NEB, 1 µL 100x BSA ...
• The environmentally-regulated interplay between local three-dimensional chromatin organisation and transcription of proVWX in E. coli

  Fatema-Zahra M. Rashid, et al., bioRxiv - Molecular Biology 2023

  Quote: ... 1.0-3.0 μg of DNA was used for a ligation reaction in a volume of 1 mL using 1.0 μL of 2000 U/μL T4 DNA Ligase (NEB) for 3C experiments ...
• Mapping temperature-sensitive mutations at a genome-scale to engineer growth-switches in E. coli

  Thorben Schramm, Vanessa Pahl, Hannes Link, bioRxiv - Systems Biology 2023

  Quote: ... The purified linear DNA was used for cloning of pTS040 by Gibson assembly (NEBuilder HiFi DNA Assembly Reaction, NEB) and electroporation of E ...
• Compact engineered human mechanosensitive transactivation modules enable potent and versatile synthetic transcriptional control

  Barun Mahata, et al., bioRxiv - Bioengineering 2023

  Quote: ... qPCR was performed using 67.5ng of gDNA for each condition in 10µl reactions using Luna Universal qPCR Master Mix (NEB, M3003E).
• Ultra-high throughput mapping of genetic design space

  Ronan W. O’Connell, et al., bioRxiv - Synthetic Biology 2023

  Quote: ... and 50 ng of gDNA was used as the template in a 25 µL reaction along with 0.25 µL of Q5 polymerase (NEB), 0.5 µL of 10mM dNTPs ...
• Synthetic Homoserine Lactone Sensors for Gram-Positive Bacillus subtilis using LuxR-type Regulators

  Min Zeng, et al., bioRxiv - Synthetic Biology 2023

  Quote: ... and terminator) was assembled in one-pot Type IIS DNA assembly reaction using BsaI-HFv2 (New England Biolabs, NEB). Transcription units to assay the sensor output contained the PQS promoter expressing the gfp gene ...
• Synthetic Homoserine Lactone Sensors for Gram-Positive Bacillus subtilis using LuxR-type Regulators

  Min Zeng, et al., bioRxiv - Synthetic Biology 2023

  Quote: ... and terminator) was assembled in one-pot Type IIS DNA assembly reaction using BsaI-HFv2 (New England Biolabs, NEB). Transcription units to assay the sensor output contained the PQS promoter expressing the gfp gene ...
• Lyssa excreta: Defining parameters for fecal samples as a rabies virus surveillance method

  Faith M. Walker, et al., bioRxiv - Pathology 2023

  Quote: ... Each 10 µL reaction contained Luna Probe One-Step RT-qPCR 4X Mix (New England Biolabs, Ipswich, MA, USA), primers (10 µM) ...
• Type IV-A3 CRISPR-Cas systems drive inter-plasmid conflicts by acquiring spacers in trans

  Fabienne Benz, et al., bioRxiv - Microbiology 2023

  Quote: ... We incubated TXTL reactions at 29 °C for 6 h and digested at 37 °C with PacI (NEB R0547S) as instructed by the provider and added water instead of PacI for the undigested control ...
• The Arabidopsis U1 snRNP regulates mRNA 3’-end processing

  Anchilie F. Mangilet, et al., bioRxiv - Plant Biology 2023

  Quote: ... the SQK-RNA002 kit (Oxford Nanopore Technologies) was used together with NEBNext® Quick Ligation Reaction Buffer (NEB B6058), T4 DNA Ligase 2M U/ml (NEB M0202) ...
• Charting functional E3 ligase hotspots and resistance mechanisms to small-molecule degraders

  Alexander Hanzl, et al., bioRxiv - Molecular Biology 2022

  Quote: ... The total isolated gDNA was processed in batches of 5 µg per PCR reaction with Q5 polymerase (NEB M0491L). One PCR reaction contained 10 µl 5x reaction buffer ...
• The epigenetic modifier DOT1L regulates gene regulatory networks necessary for cardiac patterning and cardiomyocyte cell cycle withdrawal

  Paola Cattaneo, et al., bioRxiv - Developmental Biology 2022

  Quote: ... Genotyping PCR reactions (36 amplification cycles) were performed using Taq DNA Polymerase with ThermoPol Buffer (New England Biolabs, M0267L), dNTPs from Promega (U1511 ...
• OSBP is a major determinant of Golgi phosphatidylinositol 4-phosphate homeostasis

  Colleen P. Doyle, et al., bioRxiv - Cell Biology 2024

  Quote: ... or else generated by polymerase chain reaction or gBlock synthesis (IDT) and assembled using HiFi assembly (New England Biolabs) according to the manufacturer’s instructions as shown in Table 1 ...
• High-throughput determination of RNA tertiary contact thermodynamics by quantitative DMS chemical mapping

  Bret Lange, Ricardo G. Gil, Joseph D. Yesselman, bioRxiv - Biochemistry 2024

  Quote: ... The PCR reaction was mixed by combining 25 μL of Q5 High-Fidelity DNA Polymerase (New England Biolabs #M0494S), 2 μL of the oligo pool solution ...
• Rationalizing diverse binding mechanisms to the same protein fold: insights for ligand recognition and biosensor design

  Alison C. Leonard, et al., bioRxiv - Bioengineering 2024

  Quote: ... Samples were amplified using inner primers ACL-P1060 and ACL-P1061 in a 40μl PCR reaction using Q5 Hot Start 2x Master Mix (New England Biolabs) for 20-25 cycles at an annealing temperature of 64°C ...
• Skeletal Muscle Stem Cells Modulate Niche Function in Duchenne Muscular Dystrophy through YY1-CCL5 Axis

  Yang Li, et al., bioRxiv - Cell Biology 2024

  Quote: ... Libraries were prepared by on-bead reactions using the NEB Next Ultra II DNA Library Preparation Kit (NEB, E7645S). The beads were separated on a magnetic stand ...
• Optimal trade-off between boosted tolerance and growth fitness during adaptive evolution of yeast to ethanol shocks

  Ana P. Jacobus, et al., bioRxiv - Evolutionary Biology 2024

  Quote: ... PCR reactions were performed using Phusion® high-fidelity DNA polymerase according to the manufacturer’s protocol (New Englang BioLabs). Amplified flanking recombination regions were merged with the MX cassette through Circular Polymerase Exchange Cloning into the pUC19 plasmid [67] ...
• Nanopore-based consensus sequencing enables accurate multimodal tumor cell-free DNA profiling

  Li-Ting Chen, et al., bioRxiv - Genomics 2024

  Quote: For a typical blunting reaction 5-50 ng of cfDNA are mixed with 5 μl of CutSmart 10x (NEB), 5 μl of dNTPs 1mM each ...
• Building Blocks of Understanding: Constructing a Reverse Genetics Platform for studying determinants of SARS-CoV-2 replication

  Marco Olguin-Nava, et al., bioRxiv - Microbiology 2024

  Quote: ... 30 µL of the barcoded DNA was ligated onto 2.5 µL Native Ligation Adapter (NA, ONT SQK-NBD114-96) by addition of 12.5 µL NEBNext Quick Ligation Reaction Buffer (NEB) and 5 µL high conc ...
• Temporal epigenome modulation enables efficient bacteriophage engineering and functional analysis of phage DNA modifications

  Nadiia Pozhydaieva, et al., bioRxiv - Microbiology 2024

  Quote: ... 1 µL of isolated phage T4 in Pi-Mg buffer was used as a PCR template in the first PCR with the following reaction mix: 0.125 µM each primer (Supplementary Table 2) in 1x High Fidelity Master Mix (NEB) with a total volume of 10 µl ...
• Caulobacter crescentus RNase E condensation contributes to autoregulation and fitness

  Vidhyadhar Nandana, et al., bioRxiv - Biochemistry 2023

  Quote: ... in a total reaction volume of 100 µL consisting of 50 units of T4 RNA ligase 1 (NEB #M0204S), 1mM ATP ...
• Tumor-wide RNA splicing aberrations generate immunogenic public neoantigens

  Darwin W. Kwok, et al., bioRxiv - Cancer Biology 2023

  Quote: ... a Poly(A) tailing reaction was performed for 1 hour according to the HiScribe T7 ARCA manual (NEB, E2060S). Subsequently ...