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4351 - 4400 of 7437 citations for rno mir 155 RT PCR Primer Set since 2019

• Production and characterization of virus-free, CRISPR-CAR T cells capable of inducing solid tumor regression

  Katherine P. Mueller, et al., bioRxiv - Bioengineering 2021

  Quote: ... PCR was performed according to the manufacturer’s instructions using Q5 Hot Start Polymerase (NEB) using the following program ...
• High-Throughput Developability Assays Enable Library-Scale Identification of Producible Protein Scaffold Variants

  Alexander W. Golinski, et al., bioRxiv - Bioengineering 2020

  Quote: ... PCR 1 conditions: 0.02 U/μL Q5 High-Fidelity DNA Polymerase (New England Biolabs), 1X Q5 reaction buffer ...
• Dynamic control over feedback regulation identifies pyruvate-ferredoxin oxidoreductase as a central metabolic enzyme in stationary phase E. coli

  Shuai Li, et al., bioRxiv - Bioengineering 2020

  Quote: ... 2 μL of PCR mixture was used for 10 μL KLD reaction (NEB, MA), which proceeded under room temperature for 1 hour ...
• Listeria monocytogenes utilizes the ClpP1/2 proteolytic machinery for fine-tuned substrate degradation under heat stress

  Dóra Balogh, et al., bioRxiv - Biochemistry 2021

  Quote: ... Erythromycin-sensitive strains were tested with colony PCR (OneTaq DNA polymerase, New England Biolabs) using the clpP2_KO_A and clpP2_KO_D primer pair (Table 3 ...
• Listeria monocytogenes utilizes the ClpP1/2 proteolytic machinery for fine-tuned substrate degradation under heat stress

  Dóra Balogh, et al., bioRxiv - Biochemistry 2021

  Quote: ... The ligated fragments were amplified by PCR (Phusion polymerase, HF buffer, New England Biolabs) using the clpP1_A–clpP1D and clpP2_A– clpP2_CD primer pairs (Table 2) ...
• Listeria monocytogenes utilizes the ClpP1/2 proteolytic machinery for fine-tuned substrate degradation under heat stress

  Dóra Balogh, et al., bioRxiv - Biochemistry 2021

  Quote: ... Erythromycin-sensitive strains were tested with colony PCR (OneTaq DNA polymerase, New England Biolabs) using the clpP_tag fwd and rev primer pair (Table 2 ...
• Prochlorococcus phage ferredoxin: structural characterization and electron transfer to cyanobacterial sulfite reductases

  Ian J. Campbell, et al., bioRxiv - Biochemistry 2020

  Quote: ... Plasmids were constructed by ligating PCR products amplified with Q5 polymerase (New England Biolabs) using Golden Gate assembly (87) ...
• An enhanced yeast display platform demonstrates the binding plasticity under various selection pressures

  Jiří Zahradník, et al., bioRxiv - Biochemistry 2020

  Quote: ... The template vector was removed from the PCR mixture by DpnI treatment (NEB, USA) at 37°C (1 – 2 h ...
• Strand asymmetry influences mismatch resolution during single-strand annealing

  Victoria O. Pokusaeva, et al., bioRxiv - Genomics 2021

  Quote: ... For other three libraries PCR products were digested using NheI restriction enzyme (NEB, R0131S) at 37 °C for 3 hours ...
• Endosomal Sorting Drives the Formation of Mutant Prion Endoggresomes

  Romain Chassefeyre, et al., bioRxiv - Neuroscience 2020

  Quote: ... All PCR amplifications were performed using the Phusion® High-Fidelity DNA Polymerase (NEB).
• The Rpd3-complex regulates expression of multiple cell surface recycling factors in yeast

  Konstantina Amoiradaki, et al., bioRxiv - Cell Biology 2021

  Quote: ... The Gibson assembly principle [82] of incubating homologous PCR products with Taq ligase (NEB), T5 exonuclease (NEB ...
• Protective anti-prion antibodies in human immunoglobulin repertoires

  Assunta Senatore, et al., bioRxiv - Neuroscience 2020

  Quote: Library inserts were generated by PCR using Phusion High Fidelity DNA polymerase (NEB Biolabs). The resulting HCDR3 library inserts were ligated into the base templates ...
• Protective anti-prion antibodies in human immunoglobulin repertoires

  Assunta Senatore, et al., bioRxiv - Neuroscience 2020

  Quote: Library inserts were generated by PCR using Phusion High Fidelity DNA polymerase (NEB Biolabs). The resulting HCDR3 library inserts were ligated into the base templates ...
• Correction of amyotrophic lateral sclerosis related phenotypes in induced pluripotent stem cell-derived motor neurons carrying a hexanucleotide expansion mutation in C9orf72 by CRISPR/Cas9 genome editing using homology-directed repair

  Nidaa Ababneh, et al., bioRxiv - Neuroscience 2019

  Quote: ... the reannealed PCR products were digested with T7 endonuclease 1 (T7E1, New England Biolabs). Digestion was performed using 10 unites of T7E1 enzyme and incubated for 15 minutes at 37°C ...
• Targeted gene correction and functional recovery in achondroplasia patient-derived iPSCs

  Huan Zou, et al., bioRxiv - Genetics 2021

  Quote: ... PCR was performed by using Q5 High-Fidelity DNA Polymerase (New England Biolabs, NEB). FGFR3 primers were:
• Targeted gene correction and functional recovery in achondroplasia patient-derived iPSCs

  Huan Zou, et al., bioRxiv - Genetics 2021

  Quote: ... PCR was performed by using Q5 High-Fidelity DNA Polymerase (New England Biolabs, NEB). FGFR3 primers were:
• Design, Mutate, Screen: High-throughput creation of genetic clocks with different period-amplitude characteristics

  Andrew Lezia, Nicholas Csicsery, Jeff Hasty, bioRxiv - Synthetic Biology 2021

  Quote: ... The entire plasmid was PCR amplified using Q5 DNA Polymerase (New England BioLabs Inc.) with the following degenerate primers where N indicates any base ...
• A CRISPRi-dCas9 system for archaea and its use to examine gene function during nitrogen fixation by Methanosarcina acetivorans

  Ahmed E. Dhamad, Daniel J. Lessner, bioRxiv - Microbiology 2020

  Quote: ... dCas9 with PCR amplified using Q5® High-Fidelity DNA Polymerase (New England Biolabs) with specific primers (Table S1 ...
• Predicting Individual Cell Division Events from Single-Cell ERK and Akt Dynamics

  Alan D Stern, et al., bioRxiv - Systems Biology 2021

  Quote: ... Fragments for lentiviral vector construction were generated via PCR using Q5 polymerase (NEB M0491S) and primers specific to SV40NLS-mCherry-P2A and Gly-FT2DDD-KTR-mClover (Table S1 ...
• Sequence determinants and evolution of constitutive and alternative splicing in yeast species

  Dvir Schirman, et al., bioRxiv - Systems Biology 2021

  Quote: 25 ul - Phusion High-Fidelity PCR Master Mix with HF Buffer (New England Biolabs)
• Protein context shapes the specificity of domain-peptide interactions in vivo

  Ugo Dionne, et al., bioRxiv - Systems Biology 2020

  Quote: ... The resulting PCR products were digested for 1h at 37°C with DpnI (NEB) and transformed in competent Escherichia coli MC1061 cells ...
• Common ALS/FTD risk variants in UNC13A exacerbate its cryptic splicing and loss upon TDP-43 mislocalization

  Anna-Leigh Brown, et al., bioRxiv - Neuroscience 2021

  Quote: ... Three rounds of nested PCR using Phusion HF 2x Master Mix (New England Biolabs) were used to obtain highly specific amplicons for the UNC13A cryptic ...
• Protective host-dependent antagonism among Pseudomonas in the Arabidopsis phyllosphere

  Or Shalev, et al., bioRxiv - Plant Biology 2021

  Quote: ... and i5 and i7 PCR amplification was done (Q5 polymerase; New England Biolabs, USA). Size selection and DNA purification were made using SPRI beads ...
• Characterization of mitochondrial health from human peripheral blood mononuclear cells to cerebral organoids derived from induced pluripotent stem cells

  Angela Duong, et al., bioRxiv - Neuroscience 2020

  Quote: ... PCR products were analyzed on an agarose gel and HindIII Ladder (New England Biolabs), and subsequently purified with the GeneJet PCR Purification kit (ThermoFisher) ...
• Mild and severe SARS-CoV-2 infection induces respiratory and intestinal microbiome changes in the K18-hACE2 transgenic mouse model

  Brittany Seibert, et al., bioRxiv - Microbiology 2021

  Quote: ... Secondary amplification reactions were performed using NEBNext High-Fidelity 2X PCR Master Mix (NEB) in 50 µL reaction (26 µL of 2X Mix ...
• Multiplex genomic recording of enhancer and signal transduction activity in mammalian cells

  Wei Chen, et al., bioRxiv - Genomics 2021

  Quote: ... ENGRAM plasmid and PCR product from above were digested with BsmBI (NEB, buffer 3.1) at 55°C for 1h and purified for ligation ...
• The Stickland fermentation precursor trans-4-hydroxyproline differentially impacts the metabolism of Clostridioides difficile and commensal Clostridia

  A.D. Reed, et al., bioRxiv - Microbiology 2021

  Quote: ... All PCRs of flanking regions were carried out using Phusion-HF Master Mix (NEB) according to the manufacturer’s protocol with an annealing temperature (Ta ...
• Global-scale CRISPR gene editor specificity profiling by ONE-seq identifies population-specific, variant off-target effects

  Karl Petri, et al., bioRxiv - Molecular Biology 2021

  Quote: ... All DNA amplifications were conducted by PCR with Phusion High Fidelity DNA Polymerase (NEB) unless otherwise stated ...
• Influenza A virus undergoes compartmentalized replication in vivo dominated by stochastic bottlenecks

  Katherine A. Amato, et al., bioRxiv - Microbiology 2021

  Quote: ... The oligo was amplified in 25 individual low-cycle PCRs using Q5 polymerase (NEB).The amplicons were pooled and gel purified prior to cloning into a modified PASTN plasmid using 50 individual ligation reactions ...
• The bacterial effector HopZ1a acetylates MKK7 to suppress plant immunity

  José S. Rufián, et al., bioRxiv - Plant Biology 2020

  Quote: ... All PCRs were performed using Q5 High-Fidelity DNA Polymerase (New England Biolabs, USA), unless otherwise stated ...
• SUMOylation of rice DELLA SLR1 modulates transcriptional responses and improves yield under salt stress

  Nuno M. Gonçalves, et al., bioRxiv - Plant Biology 2020

  Quote: ... The amplified PCR-product was recombined into the pDONR221 (ThermoFisher).The SUMO1SLR1 gene fusion was generated using high-fidelity PCR (Phusion DNA Polymerase; NEB) essentially as described in Atanassov et al ...
• Meta-transcriptomic analysis of virus diversity in urban wild birds with paretic disease

  Wei-Shan Chang, et al., bioRxiv - Microbiology 2020

  Quote: ... The RCA products were then purified using the Monarch PCR & DNA Cleanup Kit (NEB), then quantified using the Qubit dsDNA broad range assay ...
• Protein Targets of Inositol Pyrophosphate (5-IP₇) in the parasite Trypanosoma cruzi

  Brian S. Mantilla, et al., bioRxiv - Microbiology 2020

  Quote: ... PCRs were amplified using Q5® High fidelity DNA polymerase 2X master mix (NEB), 25 pmol of specific ultramers and 20 ng of DNA template ...
• Mechanistic insight into light-dependent recognition of Timeless by Drosophila cryptochrome

  Changfan Lin, et al., bioRxiv - Biochemistry 2021

  Quote: ... 50 μL PCR products were incubated with 1 μL DpnI enzyme (New England Biolabs) to clean up templates at 37 °C for 2.5 hours and then purified by gel-extraction following the manufacturer instructions (Cat# D2500-02 ...
• Transcriptional silencing of ALDH2 in acute myeloid leukemia confers a dependency on Fanconi anemia proteins

  Zhaolin Yang, et al., bioRxiv - Cancer Biology 2020

  Quote: ... The PCR product was end-repaired with T4 DNA polymerase (NEB; Cat. No. B02025), DNA Polymerase I ...
• Ectosome uptake by glia sculpts Caenorhabditis elegans sensory cilia

  Adrià Razzauti, Patrick Laurent, bioRxiv - Cell Biology 2021

  Quote: ... Cloning PCRs were performed using Phusion High Fidelity DNA polymerase (M0530L, New England BioLabs) and then validated by Sanger sequencing ...
• Functional tagging of endogenous proteins and rapid selection of cell pools (Rapid generation of endogenously tagged piwi in ovarian somatic sheath cells.)

  Celine Marlin Andrews, et al., bioRxiv - Cell Biology 2020

  Quote: ... PCR amplification was done using Q5 High-Fidelity DNA Polymerase (New England Biolabs, M0491). To amplify the transcript from the modified allele ...
• Molecular mechanisms underlying attenuation of live attenuated Japanese encephalitis virus vaccine SA14-14-2

  Pooja Hoovina Venkatesh, et al., bioRxiv - Cell Biology 2021

  Quote: ... The JEV NS1 gene was PCR-amplified with Deep Vent polymerase (New England Biolabs) using forward primer OSV 389 and sequential reverse primers OSV 381 ...
• Cancer-specific loss of TERT activation sensitizes glioblastoma to DNA damage

  Alexandra M. Amen, et al., bioRxiv - Cancer Biology 2021

  Quote: ... PCRs were carried out using Q5 High-Fidelity DNA polymerase (New England Biolabs, #M0491) with an annealing temperature of 70°C ...
• Perilipin 5 interacts with Fatp4 at membrane contact sites to promote lipid droplet-to-mitochondria fatty acid transport

  Gregory E. Miner, et al., bioRxiv - Cell Biology 2022

  Quote: ... all PCRs were performed using Q5 High Fidelity DNA polymerase (M0419; New England Biolabs) and restriction enzymes were from New England Biolabs ...
• Identification and characterization of the WYL BrxR protein and its gene as separable regulatory elements of a BREX phage restriction system

  Yvette A. Luyten, et al., bioRxiv - Molecular Biology 2022

  Quote: DNA substrates for gel shift assays were amplified by PCR using Q5 Polymerase (NEB) and purified using a DNA Clean and Concentrator kit (Zymo Research) ...
• A Novel and Prevalent Pathway in Microbial Selenium Metabolism

  Chase M. Kayrouz, Mohammad R. Seyedsayamdost, bioRxiv - Biochemistry 2022

  Quote: ... senC and egtD genes were PCR-amplified using Q5 High Fidelity DNA polymerase (NEB) with primers Vpa-SenC-F/R and Vpa-EgtD-F/R ...
• Opto-MASS: a high-throughput engineering platform for genetically encoded fluorescent sensors enabling all-optical in vivo detection of monoamines and opioids

  Michael Rappleye, et al., bioRxiv - Bioengineering 2022

  Quote: ... The insert and backbone were PCR amplified using Q5 polymerase (New England Biolabs (NEB) M0515 ...
• Fate and state transitions during human blood vessel organoid development

  Marina T. Nikolova, et al., bioRxiv - Developmental Biology 2022

  Quote: ... 50 ng PCR product was incubated with 2 µL 10X NEBuffer 2 (NEB, B7002S) and nuclease-free water adding up to 19 µL using the following program ...
• Opto-MASS: a high-throughput engineering platform for genetically encoded fluorescent sensors enabling all-optical in vivo detection of monoamines and opioids

  Michael Rappleye, et al., bioRxiv - Bioengineering 2022

  Quote: ... The insert and backbone were PCR amplified using Q5 polymerase (New England Biolabs (NEB) M0515 ...
• Multiple UBX proteins reduce the ubiquitin threshold of the mammalian p97-UFD1-NPL4 unfoldase

  Ryo Fujisawa, Karim P.M. Labib, bioRxiv - Molecular Biology 2022

  Quote: ... PCRs were conducted with Phusion® High-Fidelity DNA Polymerase (New England Biolabs, M0530), and amplified DNA fragments were cloned via the Gibson Assembly Cloning Kit (New England Biolabs ...
• The role of metal binding in the function of the human salivary antimicrobial peptide histatin-5

  Louisa Stewart, et al., bioRxiv - Microbiology 2022

  Quote: ... Amplicons were detected with Luna® Universal qRT-PCR Master Mix (New England Biolabs) in a CFXConnect Real-Time PCR Instrument (Bio-Rad Laboratories) ...
• An atlas of amyloid aggregation: the impact of substitutions, insertions, deletions and truncations on amyloid beta fibril nucleation

  Mireia Seuma, Ben Lehner, Benedetta Bolognesi, bioRxiv - Genomics 2022

  Quote: ... 10ng of the library were amplified by PCR (Q5 high-fidelity DNA polymerase, NEB) for 12 cycles with primers annealing to the constant regions (primers MS_01-02 ...
• Localized Cardiolipin Synthesis is Required for the Assembly of MreB During the Polarized Cell Division of Chlamydia trachomatis

  Scot P. Ouellette, et al., bioRxiv - Microbiology 2022

  Quote: ... and mreB genes were amplified by PCR with Phusion DNA polymerase (NEB, Ipswich, MA) using 10 ng C ...
• Selection of Synthetic Proteins to Modulate the Human Frataxin Function

  María Florencia Pignataro, et al., bioRxiv - Biochemistry 2022

  Quote: ... and the cDNA was amplified by PCR using Vent DNA polymerase (New England Biolabs). After DNA purification using the QIAEX II kit (QIAGEN) ...