Bio-Rad Aurum™ Total RNA 96 Kit User Manual

17

Problem

Possible Cause

Recommended Solution

Clogging of RNA

Excessive amount of

Reduce volume of

binding plate

starting material per well culture used

Incomplete mixing of lysis Mix RNA lysis solution

and alcohol solutions

and alcohol thoroughly

by pipetting up and

down

Incomplete

Pipette lysate up and

homogenization of cell

down further to reduce

lysate

lysate viscosity

Incomplete digestion with Increase duration of

lysozyme or lyticase

lysozyme or lyticase

digestion; use fresh

enzyme

Low RNA yield

Low amount of starting

Increase starting material

material

amount up to the

maximum indicated for

the specific starting

material type

Incorrect use of wash

Add the appropriate

solutions

volume of 95–100%

ethanol to the low

stringency wash solution

before initial use

Incorrect preparation

Use only the DNase

of DNase dilution

dilution solution provided

in the kit to dilute the

DNase I

Low sample eluate

See problem “Low or

volume

highly variable eluate

volumes among wells”

Inefficient elution

Preheat the elution

solution to 70°C in water

bath prior to the elution

step

Incomplete lysis

Pipet lysate up and down

further to facilitate lysis