Microvolume Measurement: How 1 uL Works
Microvolume spectrophotometers measure as little as 1 uL by compressing a liquid drop into an ultra-thin optical film between two surfaces.
측정방법
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Nucleic Acid Quantification and the A260/A280 Ratio
Measuring absorbance at 260 nm and 280 nm gives both concentration and purity of DNA and RNA samples in a single rapid scan.
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Protein Assays Compared: Bradford, BCA, Biuret, Lowry
Bradford, BCA, Biuret, and Lowry assays each convert protein concentration into a measurable color change through different chemical mechanisms and working ranges.
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ELISA: Principles and Workflow
ELISA uses enzyme-linked antibodies to detect and quantify proteins in solution, converting binding events into a measurable color change read by a microplate reader.
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Endotoxin Testing: the Kinetic Turbidimetric Method
The kinetic turbidimetric LAL method quantifies bacterial endotoxin by tracking rising absorbance over time in a microplate reader.
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Enzyme Kinetics Measurement
Enzyme kinetics measurement tracks absorbance change over time to determine reaction rates, Michaelis-Menten constants, and inhibitor effects.
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Color Analysis: ADMI and ASTA Methods
ADMI and ASTA are standardized UV-Vis methods for quantifying color in wastewater and red spices using defined absorbance measurements.
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Inline Process Measurement (PAT)
Process Analytical Technology uses inline spectroscopic probes to monitor critical quality attributes in real time during manufacturing.
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Single-Beam vs Double-Beam Spectrophotometers
Both designs measure absorbance, but they handle the reference differently. The choice affects stability, speed, and cost.