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6351 - 6400 of 7434 citations for rno mir 129 RT PCR Primer Set since 2019

• A one-tube method for rapid and reliable plant genomic DNA isolation for PCR analysis

  Wei Hu, J. Clark Lagarias, bioRxiv - Plant Biology 2020

  Quote: ... 1.5 μl of DNA extract was added to 25 μl of LongAmp Taq DNA polymerase PCR reaction mix (Cat # = M0323, New England Biolabs) following the manufacturer’s protocol ...
• Expression of fatty acyl-CoA ligase drives one-pot de novo synthesis of membrane-bound vesicles in a cell free transcription-translation system

  Ahanjit Bhattacharya, et al., bioRxiv - Synthetic Biology 2021

  Quote: ... the templates were prepared by polymerase chain reaction (PCR) amplification from corresponding plasmid constructs using Q5 DNA Polymerase Master Mix (NEB). The PCR reaction was worked up using a Qiagen PCR purification kit ...
• Elucidating the correlation between the number of TTTTGAT heptamer repeats and cholera toxin promoter activity in Vibrio cholerae O1 pandemic strains

  Arindam Naha, et al., bioRxiv - Microbiology 2021

  Quote: ... The PCR product was cloned into NdeI-SapI site of the expression vector pTXB-1 (Table 1, New England Biolabs) with a C-terminally tagged chitin binding domain (CBD ...
• Dynamic relocalization of the cytosolic type III secretion system components prevents premature protein secretion at low external pH

  Stephan Wimmi, et al., bioRxiv - Microbiology 2020

  Quote: ... Constructs with single amino acid substitutions in SctD or SctF were created by overlapping PCR using Phusion polymerase (New England Biolabs), and expressed from an arabinose controlled expression vector (pBAD).
• Mono-ADP-ribosylation by ARTD10 restricts Chikungunya virus replication by interfering with the proteolytic activity of nsP2

  Sarah Krieg, et al., bioRxiv - Microbiology 2020

  Quote: ... Linkers (5’-ACTAGTTCCGAGCTCGAG-3’) with restriction sites for SpeI and XhoI were introduced by PCR based mutagenesis using the Q5 mutagensis kit (NEB) after codon 466 of nsP2 (2EGFP ...
• Structure-guided optimization of light-activated chimeric G-protein coupled receptors

  Alexandra-Madelaine Tichy, et al., bioRxiv - Molecular Biology 2021

  Quote: ... Genes were amplified in polymerase chain reactions (PCRs) using oligonucleotides with XhoI and KpnI restriction site overhangs and digested with the respective enzymes (NEB). pcDNA3.1 (Thermo Fisher Scientific ...
• Natural transformation of the filamentous cyanobacterium Phormidium lacuna

  Fabian Nies, et al., bioRxiv - Microbiology 2019

  Quote: ... 10 mg cell samples were homogenized and lysed mechanically by micropestle and subjected to PCR with Taq Polymerase (NEB, USA). The following primers were used ...
• Depurination of colibactin-derived interstrand cross-links

  Mengzhao Xue, Kevin M. Wernke, Seth B. Herzon, bioRxiv - Microbiology 2019

  Quote: ... The DNA was isolated from the supernatant using the polymerase chain reaction (PCR) clean-up kit (New England Biolabs®) and quantified using a nanodrop ...
• Reprogramming of the apoplast metabolome of Lolium perenne upon infection with the mutualistic symbiont Epichloë festucae

  Kimberly A Green, et al., bioRxiv - Microbiology 2019

  Quote: ... Cloning and screening PCR reactions were performed using Q5 High-Fidelity DNA and One-Taq DNA polymerases (New England Biolabs (NEB), Ipswich ...
• Insight into motility-dependent pathogenicity of the zoonotic spirochete Leptospira

  Jun Xu, Nobuo Koizumi, Shuichi Nakamura, bioRxiv - Microbiology 2020

  Quote: ... and the amplified product was cloned into the PCR-generated pCjSpLe94(29) by NEBuilder HiFi DNA Assembly cloning (New England BioLabs), generating pNKLiG1 ...
• Regulation of ERK2 activity by dynamic S-acylation

  Saara-Anne Azizi, et al., bioRxiv - Biochemistry 2021

  Quote: All plasmids were constructed by Gibson Assembly from PCR products generated using Q5 Hot Start DNA Polymerase (New England Biolabs) or Phusion Polymerase (generated in-house) ...
• ETV7 regulates breast cancer stem-like cell plasticity by repressing IFN-response genes

  Laura Pezzè, et al., bioRxiv - Cancer Biology 2020

  Quote: ... Purified PCR product was inserted into pAIP backbone using HpaI and EcoRI restriction endonucleases (New England Biolabs; Euroclone, Milan, Italy). Correct cloning was checked by restriction analysis and direct sequencing (Eurofins Genomics).
• Intrinsically disordered protein biosensor tracks the physical-chemical effects of osmotic stress on cells

  Cesar L Cuevas-Velazquez, et al., bioRxiv - Cell Biology 2021

  Quote: ... The digested plasmid was mixed with the different PCR-amplified sensory domains-ORFs containing overlapping ends using the Gibson Assembly method (NEB). AtLEA4-2 ...
• Cytoplasmic innate immune sensing by the caspase-4 non-canonical inflammasome promotes cellular senescence

  Irene Fernández-Duran, et al., bioRxiv - Cell Biology 2020

  Quote: ... CASP1 and CASP4 CDS were amplified from the obtained library and cloned into the pMSCV-puro vectors The caspase-4 catalytically dead C258A pMSCV-puro vector was generated from the wild-type pMSCV-puro-CASP4 through site-directed mutagenesis by PCR using the Q5 Site-Directed Mutagenesis Kit (New England Biolabs). The CASP4 and GSDMD-targeting lentiviral vectors (pGIPZ ...
• Targeted Intracellular Degradation of SARS-CoV-2 RBD via Computationally-Optimized Peptide Fusions

  Pranam Chatterjee, et al., bioRxiv - Bioengineering 2020

  Quote: ... Respective peptide DNA coding sequences (CDS) were amplified from hACE2 via PCR and inserted using HiFi DNA Assembly Master Mix (NEB) for Gibson Assembly into the pcDNA3-SARS-CoV-2-S-RBD-Fc backbone linearized by digestion with NheI and BamHI ...
• Pathogenic Mutations in the Kinesin-3 Motor KIF1A Diminish Force Generation and Movement Through Allosteric Mechanisms

  Breane G. Budaitis, et al., bioRxiv - Biophysics 2020

  Quote: ... The construct was amplified by PCR and inserted into pSNAP-tag®(T7)-2 vector (New England Biolabs Inc. #N9181S) with a SNAPf-EGFP-6His cassette ...
• The CIP2A-TOPBP1 complex safeguards chromosomal stability during mitosis

  Mara De Marco Zompit, et al., bioRxiv - Cell Biology 2021

  Quote: ... Deletion of the residues 561-625 (ΔNES) was done by deletion PCR using Phusion® High-Fidelity DNA Polymerase (NEB), followed by DpnI digestion of the template and transformation into bacteria ...
• Atg39 selectively captures inner nuclear membrane into lumenal vesicles for delivery to the autophagosome

  Sunandini Chandra, et al., bioRxiv - Cell Biology 2021

  Quote: ... The PCR product was assembled into pFA6a-GFP-his3MX6 (Longtine et al., 1998) digested with SalI and PacI (New England BioLabs) using the Gibson Assembly Master Mix (New England BioLabs).
• Restoration of deficient DNA Repair Genes Mitigates Genome Instability and Increases Productivity of Chinese Hamster Ovary Cells

  Philipp N. Spahn, et al., bioRxiv - Cell Biology 2021

  Quote: ... and 1 μL purified total cDNA (100-200 ng) was used to amplify target genes through high-fidelity PCR (Q5, New England Biolabs). A vector backbone fragment was obtained by PCR amplification from plasmid pcDNA3.1/zeo(+ ...
• Multivalent interactions make adherens junction-cytoskeletal linkage robust during morphogenesis

  Kia Z. Perez-Vale, et al., bioRxiv - Cell Biology 2021

  Quote: The deletion and the position of the deletion on cno locus were verified by PCR (Phusion polymerase, New England Biolabs) using the primers below ...
• Meiotic budding yeast assemble bundled triple helices but not ladders

  Olivia X. Ma, et al., bioRxiv - Cell Biology 2021

  Quote: ... The extension PCR amplicons have 40 bp of homologous sequences upstream and downstream of RED1 and were amplified with Q5 polymerase (NEB). Haploid cells were transformed by the lithium acetate/ single-stranded carrier DNA/PEG4000 method [70] ...
• Caspase-1-driven neutrophil pyroptosis promotes an incomplete NETosis upon Pseudomonas aeruginosa infection

  Karin Santoni, et al., bioRxiv - Immunology 2022

  Quote: ... 700-bp sequences of the flanking regions of the selected gene were amplified by PCR with Q5 high fidelity polymerase (New England Biolabs). Then ...
• Environmental conditions define the energetics of bacterial dormancy and its antibiotic susceptibility

  L Mancini, T Pilizota, bioRxiv - Microbiology 2022

  Quote: ... Later steps included purification of the PCR products followed by restriction with the restriction enzymes AvrII and NotI (NEB, UK) and ligation with the T4 DNA ligase (Promega ...
• RNase H-based analysis of synthetic mRNA 5’ cap incorporation

  Siu-Hong Chan, et al., bioRxiv - Biochemistry 2022

  Quote: ... transcripts containing artificial 5’ UTRs were performed using PCR-amplified templates and the HiScribe T7 High Yield RNA Synthesis Kit (New England Biolabs) according to manufacturer’s instructions ...
• Illumina But With Nanopore: Sequencing Illumina libraries at high accuracy on the ONT MinION using R2C2

  Alexander Zee, et al., bioRxiv - Genomics 2022

  Quote: ... PCR enrichment of adaptor ligated DNA was performed for 9 cycles using the NEBNext Multiplex Oligos for Illumina (NEB #E7600S) kit to add Illumina dual index sequences ...
• A central protein complex essential for Invasion in Toxoplasma gondii

  Mirko Singer, et al., bioRxiv - Cell Biology 2022

  Quote: ... On both sides 50 bp of homology was added via PCR to generate the repair templates for homologous recombination using Q5 polymerase (NEB). For internal tagging ...
• BREEDIT: A novel multiplex genome editing strategy to improve complex quantitative traits in maize (Zea mays L.)

  Christian Damian Lorenzo, et al., bioRxiv - Systems Biology 2022

  Quote: ... Column-purified PCR products were cloned into the Golden Gate entry vectors via a Golden Gate reaction using BbsI (New England Biolabs). All paired gRNA entry vectors were verified by Sanger sequencing.
• “Replication stalling activates SSB for recruitment of DNA damage tolerance factors”

  Elizabeth S. Thrall, et al., bioRxiv - Biochemistry 2022

  Quote: ... or pSIM6 (ampicillin).(69) Recombineering fragments bearing approximately 50 bp length homology arms were generated by PCR amplification (Q5 polymerase, New England Biolabs) of pKD3- or pKD4-based plasmids and transformed into MG1655 pSIM5 or pSIM6 by electroporation ...
• Functional characterization of putative ecdysone transporters in lepidopteran pests

  George-Rafael Samantsidis, et al., bioRxiv - Genetics 2022

  Quote: The open reading frames of SfOatp74D (Gene ID: 118271297, 2109bp) and DmOatp74D (Gene ID: 39954, 2460bp) were PCR amplified using Phusion polymerase (NEB) from cDNA templates of 3rd instar larvae of S ...
• Functional characterization of putative ecdysone transporters in lepidopteran pests

  George-Rafael Samantsidis, et al., bioRxiv - Genetics 2022

  Quote: ... The primers used to amplify the pEIA plasmid were pEIA-Fgibson and pEIA-Rgibson (S2 Table) and the PCR reaction was performed using Phusion polymerase (NEB). The ORF of the puromycin resistance gene was amplified using Phusion polymerase and pEA-PAC as a template and the primer pair used for the PCR reaction were PAC-Fgibson-AscI/PAC-Rgibson-NcoI (S2 Table) ...
• Systematic conformation-to-phenotype mapping via limited deep-sequencing of proteins

  Eugene Serebryany, et al., bioRxiv - Biophysics 2022

  Quote: ... using 10 ng of purified plasmid as the template for each 25 μl reaction and 25 PCR cycles with the Q5 Master Mix (New England Biolabs). Amplicons from the clarified culture supernatant (“SUP” ...
• Base editor scanning charts the DNMT3A activity landscape

  Nicholas Z. Lue, et al., bioRxiv - Biochemistry 2022

  Quote: ... 100 ng DNA was used as input in a first round of PCR (25–27 cycles, Q5 hot start high-fidelity DNA polymerase, New England Biolabs) to amplify the genomic loci of interest and attach common overhangs ...
• The cellular poly(rC)-binding protein 2 prevents the early steps of hepatitis C virus virion assembly

  Sophie E. Cousineau, Selena M. Sagan, bioRxiv - Molecular Biology 2022

  Quote: ... the EcoRI to KpnI fragment was subcloned to a temporary plasmid and PCR amplified with Q5 high fidelity DNA polymerase (NEB) using the dCore-BamHI-FW (5’-TTT CTG GAT CCT TGC TGG CCC TGC TGT CCT GCA TC-3’ ...
• Optimization of NLS Composition Improves CRISPR-Cas12a Editing Rates in Human Primary Cells

  Kevin Luk, et al., bioRxiv - Molecular Biology 2022

  Quote: ... regions flanking each target site were PCR amplified using locus-specific primers bearing tails complementary to the TruSeq Illumina adapters as described previously.13 25-50ng input genomic DNA is PCR amplified with Q5 High Fidelity DNA Polymerase (New England Biolabs): (98°C ...
• Mouse Nuclear RNAi-defective 2 Promotes Splicing of Weak 5’ Splice Sites

  Matyas Flemr, et al., bioRxiv - Molecular Biology 2022

  Quote: ... A volume of cDNA corresponding to 2.5 ng of the input RNA was subjected to 35 cycles of PCR with the 2 x NEBNext Ultra II Q5 Master Mix (NEB).
• Mouse Nuclear RNAi-defective 2 Promotes Splicing of Weak 5’ Splice Sites

  Matyas Flemr, et al., bioRxiv - Molecular Biology 2022

  Quote: ... and a volume of cDNA corresponding to 5 ng of the input RNA was subjected to 30 cycles of PCR with the 2 x NEBNext Ultra II Q5 Master Mix (NEB).
• Modulating CRISPR-Cas genome editing using guide-complementary DNA oligonucleotides

  Thomas Swartjes, et al., bioRxiv - Molecular Biology 2022

  Quote: The regions of interest (supplementary Table 1) were PCR amplified (supplementary table 3) from the extracted DNA using Q5 high-fidelity DNA polymerase (NEB). Of the primers used in the PCRs (supplementary table 2 ...
• The AAA+ ATPase RavA and its binding partner ViaA modulate E. coli aminoglycoside sensitivity through interaction with the inner membrane

  Jan Felix, et al., bioRxiv - Microbiology 2022

  Quote: ... The ravA and viaA genes were PCR amplified from Escherichia coli K-12 MG1655 genomic DNA using Phusion polymerase (Biolabs). All PCR products were purified by DNA cleanup kit (Qiagen) ...
• Cut-and-Paste DNA Insertion with Engineered Type V-K CRISPR-associated Transposases

  Connor J. Tou, Benno Orr, Benjamin P. Kleinstiver, bioRxiv - Synthetic Biology 2022

  Quote: ... 50 ng of genomic DNA from genome-targeting experiments were PCR amplified with 30-cycles using Q5 High-fidelity DNA Polymerase (NEB) and primers which bind just outside of TS2 or just inside of LE ...
• Functional characterization of Atlantic salmon (Salmo salar L.) PepT2 transporters

  Francesca Vacca, et al., bioRxiv - Physiology 2022

  Quote: ... while an additional step which added 3’ A-overhangs to the slc15a2a purified PCR product was performed using Taq DNA polymerase (New England Biolabs) before cloning into pCR4-TOPO vector (Thermo Fisher Scientific) ...
• Human sialomucin CD164 is an essential entry factor for lymphocytic choriomeningitis virus

  Jamin Liu, et al., bioRxiv - Microbiology 2022

  Quote: ... The sgRNA expression cassettes were amplified from gDNA in a two-step nested PCR using Q5 High-Fidelity 2X Master Mix (NEB). For PCR-I ...
• A novel fluorescent multi-domain protein construct reveals the individual steps of the unfoldase action of Hsp70

  Satyam Tiwari, et al., bioRxiv - Molecular Biology 2022

  Quote: ... fluorophores were prepared by PCR amplification from the pTriEx-MLucV plasmid using the Q5 Site-Directed Mutagenesis Kit (New England BioLabs). The proteins were expressed and purified in a similar way to MLucV ...
• Mitochondrial genomes in Perkinsus decode conserved frameshifts in all genes

  Sebastian G. Gornik, et al., bioRxiv - Molecular Biology 2022

  Quote: ... 2.5 μl reverse transcription reactions or ∼10 ng genomic DNA were then subjected to PCR amplification by the high-fidelity Phusion polymerase (NEB) in 50 μl reactions using the primer pairs listed in Supplementary Table S1 and the following cycling program ...
• Zebrafish her3 knockout impacts developmental and cancer-related gene signatures

  Matthew R. Kent, et al., bioRxiv - Developmental Biology 2022

  Quote: ... Digested PCR products were then ligated to the digested pcs2+MCS-P2A-sfGFP plasmid using T4 DNA ligase (M0202S, NEB) in a 3:1 insert:backbone ratio ...
• Human UFSP1 is an active protease that regulates UFM1 maturation and UFMylation

  David Millrine, et al., bioRxiv - Biochemistry 2022

  Quote: ... a ~1-1.5Kb fragment that included guide-RNA target sites was PCR amplified using Q5 High-Fidelity DNA Polymerase (NEB; M0491). Primers were designed using the NCBI Primer Blast tool and are documented in the key resources table ...
• The CTP-binding domain is disengaged from the DNA-binding domain in a co-crystal structure of Bacillus subtilis Noc-DNA complex

  Kirill V. Sukhoverkov, et al., bioRxiv - Microbiology 2022

  Quote: ... The resulting PCR product was gel-purified and assembled into an NdeI-HindIII-cut pET21b using a 2x Gibson master mix (NEB). Gibson assembly was possible owing to a 23-bp sequence shared between the NdeI-and-HindIII cut pET21b backbone and the PCR amplified fragment ...
• mRNA 5′ terminal sequences drive 200-fold differences in expression through effects on synthesis, translation and decay

  Antonia M.G. van den Elzen, et al., bioRxiv - Genetics 2022

  Quote: A DNA template for in vitro transcription was generated by PCR using oligos TE122 and TE126 on plasmid pCT-TE2 and Phusion DNA polymerase (NEB) in HF buffer (Table 1) ...
• Atypical MAPK regulates translocation of GATA transcription factor in response to chemoattractant stimulation

  Jeffrey A. Hadwiger, et al., bioRxiv - Developmental Biology 2022

  Quote: ... and T492 were created through PCR mutagenesis of an intron-less version of pHC329 using the oligonucleotides (#1-14) and HiFi assembly (NEB) (Fig ...
• Structural model of microtubule dynamics inhibition by Kinesin-4 from the crystal structure of KLP-12 –tubulin complex

  Shinya Taguchi, et al., bioRxiv - Biophysics 2022

  Quote: ... with the (G4S)4-GGS linker was amplified by PCR by adding a linker sequence and inserted into the pGEX-6P vector by Hi-Fi DNA assembly (NEB).
• A distant global control region is essential for normal expression of anterior HOXA genes during mouse and human craniofacial development

  Andrea Wilderman, et al., bioRxiv - Developmental Biology 2022

  Quote: ... Clones identified as edited had the target ends amplified by PCR with high-fidelity Taq polymerase (Pfusion HF; NEB, M030) and sent for Sanger sequencing (Genewiz ...