Phosphate-buffered saline tablets (PBS, pH 7.4), and poly-l -lysine–HBr (PLL–HBr) (15–30 kDa), DMSO ≥99.9% anhydrous, sodium dodecyl sulfate (SDS) ≥98.5%, and DBCO-OEG4-NHS were purchased from Sigma Aldrich and used without further purification. Methyl-OEG4-NHS was purchased from ThermoFischer Scientific, while methyltetrazine-OEG4-NHS was purchased from Click chemistry tools. TCO-DNA (15 nt, 5′-TCO-PEG4-C5-TCGTACCATCTATCC-3′) and N3-DNA (15 nt, 5′-Azido-PEG4-C5-TCGTACCATCTATCC-3′) were obtained from Biomers, cDNA (36 nt, 5′-CGCGGTCTCAGGATACCCCCCGGATAGATGGTACGA-3′) and ncDNA (36 nt, 5′AATGCTTCTCGCGCTTTTTTTTAGACTTCGCGCGTT-3′) sequences were purchased from Eurofins Genomic. Au and SiO2 QCM chips (AT cut, 5 MHz, 14 mm diameter) were purchased from Biolin Scientific. Milli-Q water with a resistivity >18 MΩ cm was used in all experiments.
Ncdna
Manufactured by Eurofins
Sourced in Greece
NcDNA is a laboratory equipment product designed for the extraction and purification of nucleic acids. It utilizes a proprietary extraction technique to efficiently isolate DNA and RNA from a variety of sample types. The core function of NcDNA is to provide a reliable and consistent means of obtaining high-quality nucleic acid preparations for further analysis and downstream applications.
Automatically generated - may contain errors
Lab products found in correlation
Dbco oeg4 nhs, by Vector Laboratories (2 mentions)
Poly l lysine hydrobromide, by Merck Group (2 mentions)
Dimethyl sulfoxide (dmso), by Merck Group (1 mentions)
Tablets for 10 mm pbs solution, by Merck Group (1 mentions)
Methyl oeg4 nhsester, by Thermo Fisher Scientific (1 mentions)
Deuterated water, by Merck Group (1 mentions)
Naclo4, by Merck Group (1 mentions)
3 protocols using ncdna
1
DNA-Click Chemistry on Surface Biosensors
2
Functionalized DNA Hybridization Assay
Check if the same lab product or an alternative is used in the 5 most similar protocols
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Poly-l -lysine hydrobromide (MW =
15–30 kDa by viscosity), poly(sodium 4-styrenesulfonate) (average
MW = 70 kDa), D2O, and tablets for 10 mM PBS solution (pH
7.4, ionic strength of 150 mM) were obtained from Sigma-Aldrich. HCl
solution was obtained from SelectiPur. Methyl-OEG4-NHS
ester was purchased from ThermoFisher Scientific, while DBCO-OEG4-NHS was obtained from Click Chemistry Tools. The membranes
for dialysis (Spectra/Por, 6–8 kDa cutoff, diameter of 6.4
mm) were purchased from Spectrum Labs, Greece. The azide-DNA (MW,
7421 g/mol; 5′-N3-PEG4-ACCACAAGTTTATATTCAGTCAT-3′,
23 nt) was acquired fromBiomers.net GmbH (chemical structure of the linker in Figure S1 ). cDNA (complementary to the KRAS sequence, 5′-ATGACTGAATATAAACTTGTGGTAGTTGGAGCTGGTGGCGTAG-3′,
43 nt) and ncDNA (5′-CTACGCCACCTCAACCTACGCCACCTCCACCTACGCCACCTC-3′,
42 nt) were purchased from Eurofins Genomics and used as received.
15–30 kDa by viscosity), poly(sodium 4-styrenesulfonate) (average
MW = 70 kDa), D2O, and tablets for 10 mM PBS solution (pH
7.4, ionic strength of 150 mM) were obtained from Sigma-Aldrich. HCl
solution was obtained from SelectiPur. Methyl-OEG4-NHS
ester was purchased from ThermoFisher Scientific, while DBCO-OEG4-NHS was obtained from Click Chemistry Tools. The membranes
for dialysis (Spectra/Por, 6–8 kDa cutoff, diameter of 6.4
mm) were purchased from Spectrum Labs, Greece. The azide-DNA (MW,
7421 g/mol; 5′-N3-PEG4-ACCACAAGTTTATATTCAGTCAT-3′,
23 nt) was acquired from
43 nt) and ncDNA (5′-CTACGCCACCTCAACCTACGCCACCTCCACCTACGCCACCTC-3′,
42 nt) were purchased from Eurofins Genomics and used as received.
3
Biomolecular Conjugation and Characterization
Check if the same lab product or an alternative is used in the 5 most similar protocols
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Poly-l -lysine hydrobromide (MW =
15–30 kDa by viscosity), NaClO4, deuterated water,
and tablets for a 10 mM PBS solution (pH 7.4) were obtained from Sigma-Aldrich.
H2SO4 (95%) was purchased from VWR Chemical,
and HCl was obtained from SelectiPur. Methyl-OEG4-NHS ester
was obtained from Thermo Fisher Scientific, while DBCO-OEG4-NHS was obtained from Click Chemistry Tools. The membrane for dialysis
(Spectra/Por; 6–8 kDa cutoff; diameter, 6.4 mm) was purchased
from Spectrum Labs, Greece. cDNA (complementary to KRAS sequence: 43 nt, 5′-ATG ACTGAATATAAACTTGTGGTAGTTGGAGCTGGTGGCGTAG-3′)
and ncDNA (42 nt, 5′-CTACGCCACCTCAACCTA CGCCACCTCCACCTACGCCACCTC-3′)
were purchased from Eurofins Genomics and used as received. The ferrocene-labeled
DNA (23 nt; MW, 7487 g/mol; 5′-ACCACAAGTTTATATTCAGTCAT-Fc-3′)
was acquired from Biomers.net GmbH. Gold QCM chips (with a fundamental
frequency of 5 MHz) were purchased from Biolin Scientific. Silicon
p++ wafers (⟨100⟩-oriented, one-side polished,
525 ± 25 μm substrate thickness, 0.01–0.025 Ω
cm resistivity) were obtained from Okmetic Finland, while the positive
Olin 907-17 photoresist was obtained from Arch Chemicals. The PNA
probe was synthesized using a previously described procedure.59 (link)
15–30 kDa by viscosity), NaClO4, deuterated water,
and tablets for a 10 mM PBS solution (pH 7.4) were obtained from Sigma-Aldrich.
H2SO4 (95%) was purchased from VWR Chemical,
and HCl was obtained from SelectiPur. Methyl-OEG4-NHS ester
was obtained from Thermo Fisher Scientific, while DBCO-OEG4-NHS was obtained from Click Chemistry Tools. The membrane for dialysis
(Spectra/Por; 6–8 kDa cutoff; diameter, 6.4 mm) was purchased
from Spectrum Labs, Greece. cDNA (complementary to KRAS sequence: 43 nt, 5′-ATG ACTGAATATAAACTTGTGGTAGTTGGAGCTGGTGGCGTAG-3′)
and ncDNA (42 nt, 5′-CTACGCCACCTCAACCTA CGCCACCTCCACCTACGCCACCTC-3′)
were purchased from Eurofins Genomics and used as received. The ferrocene-labeled
DNA (23 nt; MW, 7487 g/mol; 5′-ACCACAAGTTTATATTCAGTCAT-Fc-3′)
was acquired from Biomers.net GmbH. Gold QCM chips (with a fundamental
frequency of 5 MHz) were purchased from Biolin Scientific. Silicon
p++ wafers (⟨100⟩-oriented, one-side polished,
525 ± 25 μm substrate thickness, 0.01–0.025 Ω
cm resistivity) were obtained from Okmetic Finland, while the positive
Olin 907-17 photoresist was obtained from Arch Chemicals. The PNA
probe was synthesized using a previously described procedure.59 (link)
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