Bio-Rad Fluorescent Assay Kits User Manual

Page 7

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2. Sambrook, J., Fritsch, E. F., and Maniatis, T., Molecular Cloning: A

Laboratory Manual, Second Edition, Cold Spring Harbor Laboratory Press,
Cold Spring Harbor, New York, 16.66 (1989).

3. Seed, B., and Sheen, J. Y., Gene, 67, 271–277 (1988).

Section 7
Additional Supplies

Catalog
Number

Product Description

VersaFluor Fluorometer

170-2402

VersaFluor Fluorometer 100/120/220

, includes a standard

cuvette holder, 100 standard cuvettes, one excitation filter, and
one emission filter

170-2420

Optical Filter Excitation

, EX360/40 (340–380 nm)

170-2421

Optical Filter Emission

, EM460/10 (455–465 nm)

VersaFluor Disposable Cuvettes

170-2415

Standard Cuvette

, 12.5 x 12.5 mm (OD) 4-sided optically clear

disposable, polycarbonate, 3.5 ml, 100

Fluoromark Microplate Fluorometer

170-6941

Fluoromark Microplate Fluorometer 120V

, includes software,

5 excitation filters (355, 390, 485, 544 nm and time-resolved filter),
and 5 emission filters (405, 460, 538, 590 nm, and time-resolved
filter)

Accessories

223-9522

Disposable Transfer Pipet

170-6963

96-Well Fluorescence Microplate

, solid black, 25

170-6964

96-Well Fluorescence Microplate

, solid black with clear bot-

toms, 25

9

Section 5
Appendix

5.1 Microplate Assay

The 4MU standard curve (Section 4.3) and ß-galactosidase assay

(Section 4.4) may be scaled down 1:10 to be used in a 96-well microplate
platform. The assay is performed directly in microtiter plates.
Fluorescence units are determined in a microplate fluorometer.

1.

Add 50 µl assay buffer (1x Reaction Buffer plus 0.6 mM MUG and
12.0 mM ß-mercaptoethanol) to each sample well.

2.

Add samples (0.2–0.4 µg of total protein).

3.

Incubate the microtiter plate for 15 minutes in a 37 °C incubator.

4.

Stop the reactions by adding 150 µl 1x Stop Buffer. Pipet up and
down to mix.

5.

Read samples in a microplate fluorometer.

5.2 Microplate Fluorometer Guidelines

Use the following guide for making measurements on the Bio-Rad

Fluoromark™. For other instruments used, refer to the instruction manu-
al regarding specific operation details.

Fluoromark settings:

Excitation filter

355 nm

Emission filter

460 nm

Gain

5

Flash

10

Section 6
References

1. Alam, J. and Cook, J., Analytical Biochemistry, 188, 245–254 (1990).

8

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