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Hi,
I am starting a huge oxford project that will generate a huge amount of nanopore sequencing runs. I have yet to start but in my preparations I am making a log of what metrics I should record and also what constitutes a failing metric from a good metric (lowest passing metric and highest passing metric).
Lib Prep:
Initial DNA input (min = 1ug, max=?)
Qubit read after Ampure
Qubit read after Myone bead elution (min=200ng, max?)
Sequencing:
How many accessible pores
Average read length
Amount of 2D reads
Amount of 1D reads
Sequencing time
Are there others?
What are the top and bottom limits to each metric?
Things to watch out for or pluggins to utilize while sequencing is happening?
Thanks!!!!
I am starting a huge oxford project that will generate a huge amount of nanopore sequencing runs. I have yet to start but in my preparations I am making a log of what metrics I should record and also what constitutes a failing metric from a good metric (lowest passing metric and highest passing metric).
Lib Prep:
Initial DNA input (min = 1ug, max=?)
Qubit read after Ampure
Qubit read after Myone bead elution (min=200ng, max?)
Sequencing:
How many accessible pores
Average read length
Amount of 2D reads
Amount of 1D reads
Sequencing time
Are there others?
What are the top and bottom limits to each metric?
Things to watch out for or pluggins to utilize while sequencing is happening?
Thanks!!!!
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