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• High-throughput investigation of genetic design constraints in domesticated Influenza A Virus for transient gene delivery

  Adam Sychla, et al., bioRxiv - Bioengineering 2024

  Quote: ... digesting with DpnI (NEB R0176L), and assembling by isothermal assembly ...
• High-throughput investigation of genetic design constraints in domesticated Influenza A Virus for transient gene delivery

  Adam Sychla, et al., bioRxiv - Bioengineering 2024

  Quote: ... qPCR reactions were set up using the Luna Universal qPCR Master Mix (NEB M3003S). Reactions included 6 µL of Luna Mastermix ...
• Thermally activated antibiotic production by probiotic bacteria for pathogen elimination

  Sourik Dey, et al., bioRxiv - Bioengineering 2024

  Quote: Q5 DNA Polymerase was used for DNA amplification and colony PCR screening (New England Biolabs, Germany). Gibson Assembly and site-directed mutagenesis was performed using the NEBuilder HiFi DNA Assembly Cloning Kit (E5520S ...
• A programmable arthritis-specific receptor for guided articular cartilage regenerative medicine

  Bonnie L. Walton, et al., bioRxiv - Bioengineering 2024

  Quote: ... This fragment was cloned into a lentiviral expression plasmid we have previously described (31) encoding the Notch1 core linked to the tTA transcription factor using NEBuilder HiFi DNA Assembly (New England Biolabs). The resultant plasmid encoded constitutive expression of CII-synNotch receptor from an EF1α promoter and production of the puromycin N-acetyl-transferase transgene via the constitutive PGK promoter for antibiotic selection ...
• High-throughput investigation of genetic design constraints in domesticated Influenza A Virus for transient gene delivery

  Adam Sychla, et al., bioRxiv - Bioengineering 2024

  Quote: cDNA of each library was generated using oAS345 (Supplemtary Note 21) and LunaScript Primer-Free RT Master Mix Kit (NEB E3025S).
• Thermally activated antibiotic production by probiotic bacteria for pathogen elimination

  Sourik Dey, et al., bioRxiv - Bioengineering 2024

  Quote: ... The bacterial pellet was then resuspended in 1X DNA/RNA protection reagent supplied with the Monarch Total RNA Miniprep Kit (NEB #T2010) (New England BioLabs, USA) and subjected to mechanical lysis using the FastPrep-24™ 5G bead beating grinder system (MP Biomedicals Germany GmbH) ...
• High-throughput investigation of genetic design constraints in domesticated Influenza A Virus for transient gene delivery

  Adam Sychla, et al., bioRxiv - Bioengineering 2024

  Quote: ... The LunaScript Primer-Free RT Master Mix Kit (NEB E3025S) was used to generate cDNA per manufacturer protocol ...
• High-throughput investigation of genetic design constraints in domesticated Influenza A Virus for transient gene delivery

  Adam Sychla, et al., bioRxiv - Bioengineering 2024

  Quote: ... All A-packaged effector plasmids were generated using an isothermal assembly reaction (NEB M5520AA) (13).
• Virus-free CRISPR knock-in of a chimeric antigen receptor into KLRC1 generates potent GD2-specific natural killer cells

  Keerthana Shankar, et al., bioRxiv - Bioengineering 2024

  Quote: ... Cleaved products were incubated with proteinase K (NEB, Ipswich, MA), A-tailed ...
• Virus-free CRISPR knock-in of a chimeric antigen receptor into KLRC1 generates potent GD2-specific natural killer cells

  Keerthana Shankar, et al., bioRxiv - Bioengineering 2024

  Quote: ... DNA circularization was performed using T4 DNA ligase (NEB, Ipswich, MA), followed by treatment with a mixture of exonucleases to remove residual linear DNA ...
• Virus-free CRISPR knock-in of a chimeric antigen receptor into KLRC1 generates potent GD2-specific natural killer cells

  Keerthana Shankar, et al., bioRxiv - Bioengineering 2024

  Quote: ... USER enzyme (NEB, Ipswich, MA) and T4 polyncucleotide was then used to treat the gap-repaired DNA ...
• Virus-free CRISPR knock-in of a chimeric antigen receptor into KLRC1 generates potent GD2-specific natural killer cells

  Keerthana Shankar, et al., bioRxiv - Bioengineering 2024

  Quote: ... PCRs were carried out using the Q5 Hot Start 2x Master Mix (NEB, Ipswich, MA) according to the manufacturer’s protocol for 30 cycles ...
• Virus-free CRISPR knock-in of a chimeric antigen receptor into KLRC1 generates potent GD2-specific natural killer cells

  Keerthana Shankar, et al., bioRxiv - Bioengineering 2024

  Quote: ... ligated with a hairpin adapter (NEB, Ipswich, MA), and treated with USER enzyme (NEB ...
• TFEB controls syncytiotrophoblast differentiation

  Meagan N. Esbin, et al., bioRxiv - Cell Biology 2024

  Quote: ChIP-seq libraries were prepared independently from two ChIP biological replicates using the NEBNext Ultra II DNA Library Prep Kit (New England Biolabs, #E6177L) according to manufacturer’s instructions with a few modifications ...
• TFEB controls syncytiotrophoblast differentiation

  Meagan N. Esbin, et al., bioRxiv - Cell Biology 2024

  Quote: ... Library samples were enriched with 11 cycles of PCR amplification in 50uL of total reaction volume (10uL 5x KAPA buffer, 1.5uL 10 mM dNTPs, 0.5uL 10 mM NEB Universal PCR primer ...
• Engineering oncogenic hotspot mutations on SF3B1 via CRISPR-directed PRECIS mutagenesis

  Mike Fernandez, et al., bioRxiv - Cancer Biology 2024

  Quote: ... All ngRNAs were cloned into pLKO.5 Puro-2A-RFP between BsmBI (New England Biolabs) cut sites ...
• Engineering oncogenic hotspot mutations on SF3B1 via CRISPR-directed PRECIS mutagenesis

  Mike Fernandez, et al., bioRxiv - Cancer Biology 2024

  Quote: ... This cassette was placed in an anti-sense orientation between two LoxP sequences and a WPRE signal and cloned into the pTwist+lenti+SFFV backbone (Twist Biosciences) between BamHI and XhoI (New England Biolabs) cut sites ...
• Engineering oncogenic hotspot mutations on SF3B1 via CRISPR-directed PRECIS mutagenesis

  Mike Fernandez, et al., bioRxiv - Cancer Biology 2024

  Quote: ... containing the K700E mutation (AAA>GAA) plus 350bp of upstream and downstream sequences was amplified using Q5 polymerase (New England Biolabs) and cloned into pUC19 (Invitrogen ...
• Engineering oncogenic hotspot mutations on SF3B1 via CRISPR-directed PRECIS mutagenesis

  Mike Fernandez, et al., bioRxiv - Cancer Biology 2024

  Quote: ... between HindIII and BamHI (New England Biolabs). The pUC19-SF3B1-K700E plasmid is also used as a double-stranded DNA (dsDNA ...
• Enhancement of colorectal cancer therapy through interruption of the HSF1-HSP90 axis by p53 activation or cell cycle inhibition

  Tamara Isermann, et al., bioRxiv - Cancer Biology 2024

  Quote: ... Equal amounts of RNA were transcribed with reverse-transcription (M-MuLV Reverse Transcriptase, NEB). Quantitative real-time PCR (qRT-PCR ...
• Engineering oncogenic hotspot mutations on SF3B1 via CRISPR-directed PRECIS mutagenesis

  Mike Fernandez, et al., bioRxiv - Cancer Biology 2024

  Quote: ... between BbsI (New England Biolabs) cut sites to produce the SF3B1 sgRNA Cas9-GFP construct ...
• Engineering oncogenic hotspot mutations on SF3B1 via CRISPR-directed PRECIS mutagenesis

  Mike Fernandez, et al., bioRxiv - Cancer Biology 2024

  Quote: ... and then incubated with 2ul of DNase I (New England Biolabs), 2ul RNase A (Invitrogen) ...
• Engineering oncogenic hotspot mutations on SF3B1 via CRISPR-directed PRECIS mutagenesis

  Mike Fernandez, et al., bioRxiv - Cancer Biology 2024

  Quote: ... between BsaI (New England Biolabs) cut sites as described26 ...
• Engineering oncogenic hotspot mutations on SF3B1 via CRISPR-directed PRECIS mutagenesis

  Mike Fernandez, et al., bioRxiv - Cancer Biology 2024

  Quote: ... Base editing sgRNA directed against the SF3B1 K700 locus was designed using BE-Designer28 and cloned into pLKO.5 Puro-2A-GFP between BsmBI (New England Biolabs) cut sites ...
• Engineering oncogenic hotspot mutations on SF3B1 via CRISPR-directed PRECIS mutagenesis

  Mike Fernandez, et al., bioRxiv - Cancer Biology 2024

  Quote: ... the hU6-pegRNA2-polyT cassette was amplified from the pU6-pegRNA-gg-acceptor backbone and ligated into ngRNA1 pLKO.5 Puro-2A-RFP between EcoRI and XhoI (New England Biolabs) to create pLKO.5-K700E-ng1+pg2-Puro-2A-RFP ...
• 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 ...
• Molecular mechanism for regulating APOBEC3G DNA editing function by the non-catalytic domain

  Hanjing Yang, et al., bioRxiv - Biochemistry 2024

  Quote: ... Uracil was removed by uracil DNA glycosylase (0.025 U/μl, New England Biolabs) at 37 °C for 15 minutes ...
• 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: ... 4 μL of t7 polymerase (New England Biolabs #M0251S), 33 μL RNase-Free water ...
• Molecular mechanism for regulating APOBEC3G DNA editing function by the non-catalytic domain

  Hanjing Yang, et al., bioRxiv - Biochemistry 2024

  Quote: ... 0.1 mg/ml recombinant albumin (New England Biolabs), and 0.1 mg/ml RNase A (QIAGEN)] ...
• LPOR and the membranes – evolutionary pathway towards prolamellar body formation

  Wiktoria Ogrodzińska, et al., bioRxiv - Biochemistry 2024

  Quote: ... Fragments were ligated together with NEBuilder HiFi DNA Assembly Kit (New England Biolabs). Then Escherichia coli DH5α competent cells were transformed with the ligation mixtures and the cells containing assembled plasmid were selected on an agar medium supplemented with 100 mg/l ampicillin ...
• LPOR and the membranes – evolutionary pathway towards prolamellar body formation

  Wiktoria Ogrodzińska, et al., bioRxiv - Biochemistry 2024

  Quote: ... and ligated together with NEBuilder HiFi DNA Assembly Kit (New England Biolabs). Escherichia coli DH5α competent cells were transformed with the ligation mixtures and the cells containing assembled plasmid were selected on an agar medium supplemented with 100 mg/l ampicillin ...
• LPOR and the membranes – evolutionary pathway towards prolamellar body formation

  Wiktoria Ogrodzińska, et al., bioRxiv - Biochemistry 2024

  Quote: ... followed by cDNA synthesis with oligoT primers (ProtoScript II, New England Biolabs). The TaPOR2 gene lacking the part coding a transit peptide and pET15b plasmid (Novagen ...
• Unravelling the glycome in human intervertebral disc degeneration: Aberrant glycosylation modulates inflammation and metabolism

  Kieran Joyce, et al., bioRxiv - Bioengineering 2024

  Quote: ... – 400 U/mL (NEB); Jack bean hexosaminidase (JBH ...
• A novel functional gene delivery platform based on a commensal human anellovirus demonstrates transduction in multiple tissue types

  Cato Prince, et al., bioRxiv - Bioengineering 2024

  Quote: ... A mastermix containing 2 mmol/L of each dNTP (NEB, Ipswich, MA), 4.5 µg of random hexamers (ThermoFisher ...
• A novel functional gene delivery platform based on a commensal human anellovirus demonstrates transduction in multiple tissue types

  Cato Prince, et al., bioRxiv - Bioengineering 2024

  Quote: ... each sample was also subjected to treatment with DpnI (NEB catalog # R0176) which selectively cleaves methylated GATC sites ...
• LeGenD: determining N-glycoprofiles using an explainable AI-leveraged model with lectin profiling

  Haining Li, et al., bioRxiv - Bioengineering 2024

  Quote: ... were each treated with a mixture of PNGase F (NEB, Boston, MA, USA) following the manufacturer’s protocol.
• Stepwise Stiffening/Softening of and Cell Recovery from Reversibly Formulated Hydrogel Double Networks

  Irina Kopyeva, et al., bioRxiv - Bioengineering 2024

  Quote: ... The resultant PCR product was reassembled into a tdTomato-containing vector via Gibson assembly (NEB) with a tdTomato insert (sequence ordered as a codon-optimized gBlock from IDT ...
• 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 ...
• Distinct regions within SAP25 recruit O-linked glycosylation, DNA demethylation, and ubiquitin ligase and hydrolase activities to the Sin3/HDAC complex

  Pratik Goswami, et al., bioRxiv - Biochemistry 2024

  Quote: ... SNAP-Capture magnetic beads (S9145S) were from NEB (Ipswich, MA). Salt Active Nuclease (SAN ...
• Cell Cycle Regulation has Shaped Budding Yeast Replication Origin Structure and Function

  Chew Theng Lim, et al., bioRxiv - Biochemistry 2024

  Quote: ... The washed beads were then washed once with LSW once before resuspending in 12 μl LSW with 600 units of micrococcal nuclease (MNase, NEB M0247S) and incubated for 2 min ...
• Structure and function of the Si3 insertion integrated into the trigger loop/helix of cyanobacterial RNA polymerase

  M. Zuhaib Qayyum, et al., bioRxiv - Biochemistry 2024

  Quote: ... coli T7Express cells (New England Biolabs) cells transformed with a pET28a expression vector containing the α ...
• Cell Cycle Regulation has Shaped Budding Yeast Replication Origin Structure and Function

  Chew Theng Lim, et al., bioRxiv - Biochemistry 2024

  Quote: ... After 30 mins the samples were placed on ice and 2 μl loading dye (Purple gel loading dye, no SDS, B7025 New England Biolabs) was added prior to loading 12 μl onto a 1.5% 15 x 15 cm 100 ml 0.5X TB agarose gel ...
• Structure and function of the Si3 insertion integrated into the trigger loop/helix of cyanobacterial RNA polymerase

  M. Zuhaib Qayyum, et al., bioRxiv - Biochemistry 2024

  Quote: ... coli T7Express cells (New England Biolabs) as the N-terminal His6-tagged protein ...
• Cell Cycle Regulation has Shaped Budding Yeast Replication Origin Structure and Function

  Chew Theng Lim, et al., bioRxiv - Biochemistry 2024

  Quote: ... was 5’ end labelled in a final volume of 10 μl using 0.6 μl T4 PNK (10U/μl, M0201 New England Biolabs) with 2 μl gamma 32P ATP 3000Ci/mmol (SRP-301 Hartmann) ...
• Structure and function of the Si3 insertion integrated into the trigger loop/helix of cyanobacterial RNA polymerase

  M. Zuhaib Qayyum, et al., bioRxiv - Biochemistry 2024

  Quote: ... 13 nt long RNA was radiolabelled at the 5’-end with [γ-32P] ATP and T4 Polynucleotide kinase (New England Biolabs) prior to complexes assembly ...
• Late consolidation of rRNA structure during co-transcriptional assembly in E. coli by time-resolved DMS footprinting

  Yumeng Hao, et al., bioRxiv - Biochemistry 2024

  Quote: ... 4SU-labeled RNA (100 µg) was biotinylated with HPDP-biotin (cat. 21341, ThermoScientific) and captured on 150 µL of streptavidin magnetic beads (NEB) per RNA sample ...
• Structural basis for Retriever-SNX17 assembly and endosomal sorting

  Amika Singla, et al., bioRxiv - Biochemistry 2024

  Quote: ... Isolated MBP-tagged VPS26C was purified using Amylose beads (New England Biolabs) and eluted using 20 mM Tris pH 8.0 ...
• Cryo-EM structure of the tetra-phosphorylated R-domain in Ycf1 reveals key interactions for transport regulation

  Rodolpho S. A. de Carvalho, et al., bioRxiv - Biochemistry 2024

  Quote: ... the concentrated protein at 3 mg/mL was incubated with c-AMP Protein Kinase A PKA (NEB) (molar ratio of 40:1 ...
• Viral proteins activate PARIS-mediated tRNA degradation and viral tRNAs rescue infection

  Nathaniel Burman, et al., bioRxiv - Biochemistry 2024

  Quote: ... and 1 mM DNA oligo in T4 polynucleotide kinase buffer (NEB). This mixture was then incubated at 37°C for 1 hour ...
• Viral proteins activate PARIS-mediated tRNA degradation and viral tRNAs rescue infection

  Nathaniel Burman, et al., bioRxiv - Biochemistry 2024

  Quote: ... The ATP and ADP makers were created using T4 polynucleotide kinase (NEB). T4 PNK mixed with 128 µM ATP supplemented with 10 nM [α-32 P]-ATP ...