Flowcell installation | Second-generation sequencing

Second-generation sequencing > Flowcell installation

Flowcell installation

Equipment and consumables
Installation
Focusing
Notes

Comments

NB! post-PCR operation.

Equipment and consumables

check that data collected from the previous run are satisfactory;
empty the waste canister;
prepare:
- two glass beakers for washing tubing;
- three glass beakers for O-ring wash:
  
  H₂O initial water wash
  
  70% ethanol ethanol wash
  
  H₂O final water wash
aspiration pump;
waste bin for excess of 1x Instrument Buffer;
2ml tubes for control of deposition;
screwdrivers for bolts & for deposition chamber;
place, where to put the old assembly (storage chamber or PP-container for slides);
plastic box with water for plastic parts of deposition chambers;
plastic box for metal parts of deposition chambers;

Installation

launch ICS:
- remove previous run: "clear";
- if necessary, unlock doors;
- click on reagent chiller button to select "Cooling" (bottom middle);
create a new run (see "QC-run" or "35-bp run" or PE-run");
prepare instrument FlowCell:
- insert paper towels under the FC chambers;
- in ICS: Clear Flowcell & Yes;
- open FlowCell chamber;
- remove old slide assembly & put it in a appropriate place (work fast to prevent drying of slides);
- clean O-rings:
    •   remove O-ring;
    •   THOROUGHLY check integrity of O-ring;
    •   wash O-ring sequentially by water, 70% ethanol & water again;
- clean FlowCell chamber:
    •   remove excess of the liquid from FlowCell chamber (aspiration & paper towel);
    •   clean FlowCell chamber with water and 70% ethanol;
    •   carefully remove all liquid;
- put few drops of 1x Instrument buffer on FlowCell chamber & install O-ring (DO NOT TWIST O-ring!);
- check evenness of O-ring by finger, re-install it if necessary;
open a new slide:
- remove adhesive paper from holes;
- add 1x Instrument Buffer to the reservoir of deposition chamber;
- with 1ml pipettor aspirate SLOWLY the Deposition Buffer from the well & put it into prepared 2ml tube (later control the absence of beads on magnetic stand);
- diagonally loosen screws;
- open assembly;
- put additional 1x Instrument Buffer on the top of the slide;
install slide:
- click "Load Flowcell" button (DO NOT click "OK");
- find orientation of the slide carrier;
- QUICKLY pour off the excess of the 1x Instrument Buffer & install slide carrier (work fast to prevent drying of slides);
- gradually tighten two bolts;
- check, that liquid does not move when tightening;
- aspirate the excess of liquid from the FlowCell holder;
- wipe first with wet and then with dry paper towel the glass surface;
- rotate FlowCell up & lock;
- click OK in the ICS dialog box;
- wait, until FolwCell is loaded & open FlowCell down;
- check, that there are not to much bubbles (otherwise repeat "Load Flowcell" command);
- aspirate excess of the liquid from FlowCell block, liquid trap & clean it with 70% ethanol;
clean glass slide:
- 2x one-way wiping with lens-cleaning tissue slightly moistened with water;
- 3x one-way wiping with lens-cleaning tissue slightly moistened with ethanol;
- rotate FlowCell up & lock;
- repeat "Load Flowcell" command and check for leaking;

Focusing

find the old "average distance" in the file C:/Documents and Settings/All Users/Application Data/Applied Biosystems/discovery/imager_local (link on the desktop);

old focus: ____________ ____________ ____________ ____________
lock doors of the instrument;
menu: Window > Imaging System;
select the following parameters (repeat the already selected):
- proper flowcell number in "Show FlowCell";
- "Gain": 1;
- WL (white light) in "Filter status" box;
- "2" in "Nosepiece Status";
- "2" in "Prism Status";
menu: View > Stage template & select proper *.STG file:
- 1 well: mask_1_spot
- 4 wells: mask_4_spot
- 8 wells: mask_8_spot
move green-box cursor into upper-left corner;
in "Focus Status" go to "old focus" value;
click "AutoExposure";
manually find a focus position (with 500 accuracy for EXTREME values):
- acquire;
- check image & correct focus distance;

NB! reinstall the glass if the "MAX-MIN" range exceeds 5000

Z=(MIN+MAX)/2=________________

     _________________               _________________

                         _________________

     _________________               _________________

calculate the (MIN+MAX)/2 value;
menu: Options > Focusing:
- switch off "Use default focusing range";
- insert: Z Min = Z-5000; Z Max = Z+5000;
- "Save to Flowcell" and approve the FlowCell number;
repeat §§3-11 for the flowcell 2;
check new settings:
- close all windows;
- open ICS again;
- check that new settings are in the imager_local file;
- menu: Window > Imaging System;

Notes

never scrape surfaces with paper towels. To remove liquid: press paper towel, wait few seconds and remove;

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Last modification: 01/12/08

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