Rob McMinn iSeq Run (loc_ad2)
02-04-2022 Illumina agreed there was likely a consumables problem. They are sending a replacement cartridge next week.
This r-script was used to transform this LIMS report to this demux key.
iSeq Global Metrics
%Q30 Read 1 | 78.8 |
%Q30 Read 2 | 75.2 |
%Clusters PF | 39 |
%Occupancy | 90.2 |
%Clusters Passing Filter is concerning. We will reach out to Illumina.
Sample Processing
Plate: RMJan22
NOTE: Plate sequenced for 16S only but ITS was prepped up until MagBead. No MagBead clean up was completed on ITS but is available if client would like to sequence for ITS in the future.
MasterMix (make for 4 plates in 5 mL tube)
ul/rxn | Reagent | # of rxns | ul needed |
|---|---|---|---|
3 | 5X Kapa HiFi Buffer | 80 | 330 |
0.45 | 10M dNTPs | 80 | 50 |
0.3 | Kapa HiFi HotStart DNA Pol | 80 | 33 |
7.25 | HPLC H2O | 80 | 797 |
11 | Total Volume | 80 | 1210 |
Add 11 ul to each well of a hard shell, full skirt plate. Seal with bubble strips and store in refrigerator until needed label “NovaSeq4 PCR”. (If doing manually, one needs 2 ul of template and 2 ul of the primers).
Plate | 16S MID |
|---|---|
RMJan22 | 16S0A4 |
16S0B4 |
*ITS plates PCR’d but did not continue to MagBead clean up.
Run on Thermocycler Program GSAF36:
Temp C | Cycles | Time |
|---|---|---|
95* | 1X | 3:00* |
98 | 36X | 0:30 |
62 | 36X | 0:30 |
72 | 36X | 0:30 |
72 | 1X | 5:00 |
4 | 1X | 0:00 |
MagBead Cleanup (16S Only):
Some plates were cleaned up using the Nimbus platform protocol “AxyPrep MagBead PCR1 No MM”
Manually, it was done:
Equilibrate Beads to room Temperature
Add 24 ul of MagBeads to each well and 15 ul of replicate to same well of replicate
Pipette mix up and down 10 times.
Incubate at RT for 5 minutes
Secure plate on magnet plate; incubate at RT for 5 minutes (until wells are clear)
Remove 65 ul from each well; keep tips to left or right depending on the column to avoid bead pellet.
Add 100 ul Fresh 80% EtOH to each well. Incubate 30 seconds. Remove 100 ul from each well
Add 100 ul Fresh 80% EtOH to each well. Incubate 30 seconds. Remove 100 ul from each well
Reaspirate from each well to assure maximum EtOH removal
Allow plate to air dry for 7 minutes.
Remove sample plate from magnet plate.
Add 40 ul TE; pipette mix 10+ times. Incubate 2 minutes at RT.
Place sample plate back on magnet for 5 minutes or until all wells are cleared.
Transfer 40 ul to labeled transparent plate (Plate name_PCR_MIDs)
qPCR
Pool 2uL from each well into a single pool. Make 1:10000 dilution of RMJan22 Pool and run in triplicate on qPCR.
Add 16 ul of Illumina Library Quantification MasterMix to each well:
ul/rxn | Reagent | # of rxns | ul needed |
|---|---|---|---|
10 ul | KAPA SYBR FAST qPCR MM (2X) | 50 | 500 |
2 ul | Primer Premix (10X) | 50 | 100 |
4 ul | Ultra Pure Water | 50 | 200 |
16 ul | Total Volume | 50 | 800 |
Add 4 ul of template, pool, or standards to each well:
| 1 | 2 | 3 | 4 | 5 | 6 | 7 | 8 | 9 | 10 | 11 | 12 |
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A |
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| NTC | NTC | NTC |
B |
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| 0.0002 pM Std | 0.0002 pM Std | 0.0002 pM Std |
C |
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| 0.002 pM Std | 0.002 pM Std | 0.002 pM Std |
D |
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| 0.02 pM Std | 0.02 pM Std | 0.02 pM Std |
E |
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| 0.2 pM Std | 0.2 pM Std | 0.2 pM Std |
F |
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| 2 pM Std | 2 pM Std | 2 pM Std |
G |
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| 20 pM Std | 20 pM Std | 20 pM Std |
H |
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Results:
Average results for the following plates:
Full result report can be viewed below:
iSeq Run:
Dilute to 1 nM based off qPCR results. qPCR results are in pM, but 1:1000 dilution used. The results are effectively in nM for pool.
100/Results = ul of Pool to Add
100/4.98 = 20uL of Pool to Add
100 - uL of Pool to Add = ul of “10 mM Tris 8.5” to Add
100- 20 = 80uL of 10mM Tris 8.5
Dilute 1 nM full pool to loading concentration of 50 pM:
Add 5 ul 1 nM Pool to 85 ul “10 mM Tris 8.5” and 10 ul 50 pM PhiX
Remove iSeq 100 i1 Flow Cell from refrigerator 5’s crisper drawer and open white foil pack and allow to equilibrate to RT for 10-15 minutes.
Open “iSeq 100 i1 Reagent Cartridge v2”. Turn on iSeq100
Click on “Sequence”. Watch Video. Do what video tells you to do. Follow on screen instructions until run starts.
The sequencing run showed poor global statistics:
Statistic | Percentage |
|---|---|
%Q30 Read 1 |
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%Q30 Read 2 |
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%Clusters PF |
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%Occupancy |
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A double check of the 1nM pool dilution created for sequencing revealed it was actually 4.98 nM. We will repeat sequencing run.