Flow Cell Wash Kit (EXP-WSH004 or EXP-WSH004-XL)
MinION: Protocol
Flow Cell Wash Kit (EXP-WSH004 or EXP-WSH004-XL) V WFC_9120_v1_revQ_08Dec2020
For Research Use Only
FOR RESEARCH USE ONLY
Contents
Introduction to the protocol
Flushing, reloading or storing a flow cell
概要
For Research Use Only
1. Overview of the protocol
Introduction to the Flow Cell Wash Kit
The Flow Cell Wash Kit allows sequential runs of multiple sequencing libraries on the same flow cell. It works by flushing out and digesting the first library, refreshing the system for a subsequent library to be loaded. This procedure provides the opportunity to utilise the same flow cell a number of times, maximising the available run time, particularly for cases where less data per library is required. Following the wash step, Storage Buffer can be introduced into the flow cell, allowing storage of the flow cell at 4-8°C. The Flow Cell Wash Kit is compatible with Q-Line, R9.4.1 and R10.4.1 flow cells.
The nuclease digests DNA library and for effective removal from the flow cell before loading a new library, we recommend removing the waste buffer from the waste ports after each flush step. This is to ensure there is no nuclease in the waste channel that may diffuse through the flow cell during sequencing. To further improve flow cell output after a wash, we recommend pipetting slowly during flushing steps by either twisting the pipette wheel down slowly or pressing the plunger down slowly.
Please note, although the wash procedure should remove 99.9% of the library, some residual DNA may remain on the flow cell. For this reason, we recommend to barcode your libraries when used in conjunction with the Flow Cell Wash Kit, to ensure that reads from different libraries can be separated from each other.
Successful deconvolution of DNA reads has been demonstrated in Oxford Nanopore's internal development:
Figure 1. A sample with four barcodes was sequenced and washed using EXP-WSH004 before a sample with four different barcodes was loaded. This was repeated for a third sequencing run.
For users who wish to use barcoding to run multiple libraries at one time rather than washing the flow cells, please see the barcoding kits we have available in the chemistry technical document.
The Flow Cell Wash Kit is can also be used with our RNA flow cells to flush out RNA libraries, but will not remove RNA-related blocking and restore nanopores.
Nuclease activity of the Flow Cell Wash Kit
The Flow Cell Wash Kit contains DNase I, that is used to digest any remaining DNA library on a flow cell. Once the library is removed, the flow cell can be re-used immediately or stored for later use.
During sequencing, an accumulation of pores in the “unavailable" state (Figure 2) may be observed, causing the rate of data acquisition to decline as fewer pores are available to accept and sequence strands. We have demonstrated that in these circumstances, pores can be reverted to the “active pore” state by pausing sequencing and washing the flow cell with the DNase I in the Flow Cell Wash Kit. In Figure 2, the astrisks indicate where sequencing has been paused and the flow cell washed. Note: If the sequencing run is paused in MinKNOW for the flow cell wash, you will only see the restoration of sequencing pores after a new pore scan has been performed.
The wash step is recommended where sequencing channels are lost to the “unavailable” state (Figure 2). In circumstances where channels have been lost by other means, for example “saturated”, the wash step is not effective at reverting channels to the “active pore” state. If your sample is not known to block and cause saturation of the flow cell, we recommend loading a fresh library on a new flow cell. If you do not have excess library to load on a new flow cell, you can recover the library and reload on a new flow cell following method 1 of the Library recovery from flow cells protocol.
Figure 2. Pore states observed on a flow cell before and after wash steps are performed. A flow cell has been loaded with a sequencing library that has resulted in an accumulation of pores in the “unavailable” state, leading to a decrease in the rate of data acquisition. The red asterisks indicate when a wash step has been performed. A significant number of the pores that had been lost to the “unavailable” state have reverted to the “Pore available” state and are available for sequencing once again.
In experiments where output is limited by the increase in pores in the “unavailable” state, we have shown that output can be improved by performing several wash steps over the lifetime of a flow cell. Figure 3 shows the output obtained from a PromethION Flow Cell loaded with a library of DNA extracted from chicken - Gallus gallus, and a MinION Flow Cell loaded with a library of DNA extracted from a type of Japense ricefish - Oryzias latipes, where unavailable pores increased over the course of the experiment, and so flow cell washes were performed to unblock the pores (Figure 3). In each case, the use of multiple washes allowed for an improvement of the output from the flow cell, without any compromise in observed read length (Figure 4).
Figure 3. Throughput observed from Gallus gallus and Oryzias latipes libraries run on a PromethION Flow Cell and a MinION Flow Cell, respectively. The arrows indicate the timing of each wash step: wash steps were performed at the point where the rate of data acquisition started to slow due to the accumulation of “recovering” pores. In each case, output is more than doubled from the point of the first wash.
Figure 4. Effective inactivation of the DNase I prevents read length deterioration in the experiments after a nuclease wash is performed. In this example, the read length of the Gallus gallus library was recorded before the first wash (load #1) and then again after the first and second washes (load #2 and #3, respectively). No decrease in read length is observed.
2. Equipment and consumables
材料
- Flow Cell Wash Kit (EXP-WSH004) or Flow Cell Wash Kit XL (EXP-WSH004-XL)
- Flow cell priming reagents available in your sequencing kit or in the following kits:
- Sequencing Auxiliary Vials V14 (EXP-AUX003)
- Flow Cell Priming Kit (EXP-FLP004)
装置
- P1000 ピペット及びチップ
- P20 ピペットとチップ
- アイスバケツ(氷入り)
Reloading a library
Additional buffers are required for reloading a library following the washing of a flow cell. These can be found in the one of the following expansion kits:
Sequencing Auxiliary Vials V14 (EXP-AUX003). This expansion contains vials of Sequencing Buffer (SB), Elution Buffer (EB), Library Solution (LIS), and Library Beads (LIB) with Kit 14 flow cell priming reagents: Flow Cell Flush (FCF) and Flow Cell Tether (FCT). This expansion is only compatible with our Kit 14 chemistry e.g. SQK-LSK114.
Flow Cell Priming Kit (EXP-FLP004). This expansion contains both Kit 14 flow cell priming reagents required: Flow Cell Flush (FCF) and Flow Cell Tether (FCT). This expansion is only compatible with Kit 14 chemistry.
For our previous chemistries:
Sequencing Auxiliary Vials expansion (EXP-AUX001). This expansion contains vials of Elution Buffer (EB), Sequencing Buffer (SQB), and Loading Beads (LB), additional to those found in DNA sequencing kits for our Kit 9 chemistry.
Sequencing Auxiliary Vials expansion (EXP-AUX002). This expansion contains vials of Sequencing Buffer II (SBII), Elution Buffer (EB), Loading Solution (LS), and Loading Beads II (LBII), additional to those found in Kit 10 and 11 chemistry, such as:
- Kit 10 e.g. SQK-LSK110
- Kit 11 e.g. SQK-PCS111
- Flow Cell Priming Kit (EXP-FLO002). This expansion contains both flow cell priming reagents required: Flush Buffer (FB) and Flush Tether (FLT). This expansion is compatible with Kit 9, 10 and 11 chemistry.
Flow Cell Wash Kit (EXP-WSH004) contents
| Contents | Volume (µl) | No. of tubes | No. of uses |
|---|---|---|---|
| Wash Mix (WMX) | 15 | 1 | 6 |
| Wash Diluent (DIL) | 1,300 | 2 | 6 |
| Storage Buffer (S) | 1,600 | 2 | 6 |
- Wash Mix (WMX) contains DNase I.
- Wash Diluent (DIL) contains the exonuclease buffer that maximises activity of the DNase I.
- The Storage Buffer allows flow cells to be stored for extended periods of time.
Flow Cell Wash Kit XL (EXP-WSH004-XL) contents
| Name | Acronym | Fill volume per vial (µl) | Cap colour | No. of vials | No. of uses |
|---|---|---|---|---|---|
| Wash Mix | WMX | 150 | Brown | 1 | 48 |
| Wash Diluent | DIL | 20,000 | White cap, brown stripe | 1 | 48 |
| Storage Buffer | S | 25,000 | White cap, yellow stripe | 1 | 48 |
- Wash Mix (WMX) contains DNase I.
- Wash Diluent (DIL) contains the exonuclease buffer that maximises activity of the DNase I.
- The Storage Buffer allows flow cells to be stored for extended periods of time.
Flow Cell Priming Kit (EXP-FLP004) contents
| Name | Acronym | Cap colour | No. of vials | Fill volume per vial (μl) |
|---|---|---|---|---|
| Flow Cell Flush | FCF | 6 | Clear cap, light blue lable | 8,000 |
| Flow Cell Tether | FCT | 1 | Purple | 200 |
Sequencing Auxiliary Vials V14 (EXP-AUX003) contents
| Name | Acronym | Cap colour | No. of vials | Fill volume per vial (μl) |
|---|---|---|---|---|
| Elution Buffer | EB | Black | 2 | 500 |
| Sequencing Buffer | SB | Red | 2 | 700 |
| Library Solution | LIS | White cap, pink label | 2 | 600 |
| Library Beads | LIB | Pink | 2 | 600 |
| Flow Cell Flush | FCF | Light blue label | 2 | 8,000 |
| Flow Cell Tether | FCT | Purple | 2 | 200 |
3. Flushing a MinION/GridION Flow Cell
材料
- Flow Cell Wash Kit (EXP-WSH004) or Flow Cell Wash Kit XL (EXP-WSH004-XL)
装置
- P1000 ピペット及びチップ
- P20 ピペットとチップ
- アイスバケツ(氷入り)
Preparation to run the washing procedure
- This protocol assumes that the flow cell has already had a DNA/RNA library run on it
- The aim is to remove most of this initial library from the flow cell
- The Wash Kit contains all solutions required for removal of the initial library
- Data acquisition in MinKNOW should be stopped (if loading a new library or storing the flow cell), or paused (if loading more of the same library after the wash)
- After the flow cell has been washed, a new library can be loaded or the flow cell can be stored at 4°C
ヒント
We recommend keeping the light shield on the flow cell during washing if a second library will be loaded straight away.
If the flow cell is to be washed and stored, the light shield can be removed.
重要
A P1000 pipette must be used for all flushing steps to create a seal with the flow cell ports.
Place the tube of Wash Mix (WMX) on ice. Do not vortex the tube.
Thaw one tube of Wash Diluent (DIL) at room temperature.
Mix the contents of Wash Diluent (DIL) thoroughly by vortexing, then spin down briefly and place on ice.
In a fresh 1.5 ml Eppendorf DNA LoBind tube, prepare the following Flow Cell Wash Mix:
| Reagent | Volume per flow cell |
|---|---|
| Wash Mix (WMX) | 2 μl |
| Wash Diluent (DIL) | 398 μl |
| Total | 400 μl |
Mix well by pipetting, and place on ice. Do not vortex the tube.
Stop or pause the sequencing experiment in MinKNOW, and leave the flow cell in the device.
重要
It is vital that the flow cell priming port and SpotON sample port are closed before removing the waste buffer to prevent air from being drawn across the sensor array area, which would lead to a significant loss of sequencing channels.
Remove the waste buffer, as follows:
- Close the priming port and SpotON sample port cover, as indicated in the figure below.
- Insert a P1000 pipette into waste port 1 and remove the waste buffer.
Note: As both the priming port and SpotON sample port are closed, no fluid should leave the sensor array area.
Slide the flow cell priming port cover clockwise to open.
重要
フローセルからバッファーを引き上げる際には注意してください。20~30μl以上は除去せず、ポアのアレイ全体が常にバッファーで覆われていることを確認して下さい。アレイに気泡が入ると、ポアに不可逆的なダメージを与える可能性があります。
After opening the priming port, check for a small air bubble under the cover. Draw back a small volume to remove any bubbles:
- Set a P1000 pipette to 200 µl.
- Insert the tip into the flow cell priming port.
- Turn the wheel until the dial shows 220-230 µl, or until you can see a small volume of buffer/liquid entering the pipette tip.
- Visually check that there is continuous buffer from the flow cell priming port across the sensor array.
Slowly load 200 µl of the prepared flow cell wash mix into the priming port, as follows:
- Using a P1000 pipette, take 200 µl of the flow cell wash mix
- Insert the pipette tip into the priming port, ensuring there are no bubbles in the tip
- Slowly twist the pipette wheel down to load the flow cell (if possible with your pipette) or push down the plunger very slowly, leaving a small volume of buffer in the pipette tip.
- Set a timer for a 5 minute incubation.
Once the 5 minute incubation is complete, carefully load the remaining 200 µl of the prepared flow cell wash mix into the priming port, as follows:
- Using a P1000 pipette, take the remaining 200 µl of the flow cell wash mix
- Insert the pipette tip into the priming port, ensuring there are no bubbles in the tip
- Slowly twist the pipette wheel down to load the flow cell (if possible with your pipette) or push down the plunger very slowly, leaving a small volume of buffer in the pipette tip.
Close the priming port and wait for 1 hour.
重要
It is vital that the flow cell priming port and SpotON sample port are closed before removing the waste buffer to prevent air from being drawn across the sensor array area, which would lead to a significant loss of sequencing channels.
Remove the waste buffer, as follows:
- Ensure the priming port and SpotON sample port covers are closed, as indicated in the figure below.
- Insert a P1000 pipette into waste port 1 and remove the waste buffer.
Note: As both the priming port and SpotON sample port are closed, no fluid should leave the sensor array area.
最終ステップ
Follow one of the two options described in the next steps of the protocol.
- Run a second library on the flow cell straight away
- Store the flow cell for later use
4. To run a second library on a MinION/GridION Flow Cell straight away
材料
- Flow Cell Wash Kit (EXP-WSH004) or Flow Cell Wash Kit XL (EXP-WSH004-XL)
- Flow cell priming reagents available in your sequencing kit or in the following kits:
- Sequencing Auxiliary Vials V14 (EXP-AUX003)
- Flow Cell Priming Kit (EXP-FLP004)
装置
- P1000 ピペット及びチップ
- P20 ピペットとチップ
- アイスバケツ(氷入り)
重要
The sequencing reagents outlined in this method are for our most recent V14 chemisty.
If using a previous version of our chemistry or a kit with specific sequencing reagents, please ensure you are using the correct sequencing reagents for your flow cell.
ヒント
The buffers used in this process are incompatible with conducting a Flow Cell Check prior to loading a subsequent library. However, the first pore scan once a sequencing run has started will report the number of nanopores available.
重要
A P1000 pipette must be used for all flushing steps to create a seal with the flow cell ports.
Sequencing Buffer(SB)、Library Beads(LIB)またはLibrary Solution(LISを使用する場合のみ)、Flow Cell Tether(FCT)およびFlow Cell Flush(FCF)を室温で融解してから、ボルテックスで混合します。その後、スピンダウンして氷上で保存します。
重要
MinION R10.4.1フローセル(FLO-MIN114)での最適なシークエンス性能と出力向上のために、フローセルのプライミングミックスに最終濃度0.2 mg/mlでBovine Serum Albumin (BSA) を添加することを推奨します。
(注: その他のアルブミンの種類(組換えヒト血清アルブミンなど)の使用は推奨しません。
To prepare the flow cell priming mix with BSA, combine Flow Cell Flush (FCF) and Flow Cell Tether (FCT), as directed below. Mix by pipetting at room temperature.
| Reagent | Volume per flow cell |
|---|---|
| Flow Cell Flush (FCF) | 1,170 µl |
| Bovine Serum Albumin (BSA) at 50 mg/ml | 5 µl |
| Flow Cell Tether (FCT) | 30 µl |
| Total volume | 1,205 µl |
フローセルのプライミングポートカバーを時計方向にスライドさせ、プライミングポートを開きます。
重要
フローセルからバッファーを引き上げる際には注意してください。20~30μl以上は除去せず、ポアのアレイ全体が常にバッファーで覆われていることを確認して下さい。アレイに気泡が入ると、ポアに不可逆的なダメージを与える可能性があります。
プライミングポートを開けた後に、カバーの下に小さな気泡がないかを確認して下さい。気泡を取り除くために少量の液を引き上げます。
- P1000ピペットを200 µ Lに設定して下さい。
- ピペットの先端をプライミングポートに差し込みます。
- 目盛りが220-230 ulと表示されるまでダイヤルを回して、20-30 ulを吸い上げるか、少量のバッファーがピペットの先端に入るのが見えるまでダイヤルを回します。
(注: プライミングポートからセンサーアレイ全体にバッファーがあることを確認してください。
Slowly load 800 µl of the priming mix into the priming port, as follows:
- Using a P1000 pipette, take 800 µl of the priming mix
- Insert the pipette tip into the priming port, ensuring there are no bubbles in the tip
- Slowly twist the pipette wheel down to load the flow cell (if possible with your pipette) or push down the plunger very slowly, as illustrated in the video above, leaving a small volume of buffer in the pipette tip.
重要
It is vital to wait five minutes between the priming mix flushes to effectively remove the nuclease.
Close the priming port and wait five minutes.
During this time, prepare the library for loading by following the steps below.
Library Beads(LIB)の液をピペッティングすることで十分に混合して下さい。
重要
Library Beads(LIB)チューブにはビーズの懸濁液が入っています。これらのビーズはすぐに沈殿するので、使用直前に混合することが重要です。
ほとんどのシーケンス実験にはLibrary Beads (LIB)の使用を推奨します。しかし、より粘性の高いライブラリーにはLibrary Solution(LIS)を使ってください。
In a new tube, prepare the library for loading according to the "Priming and loading the MinION and GridION Flow Cell" section of the suitable protocol to ensure you are using the correct reagents and volumes.
For Kit 14 chemistry:
| Reagent | Volume per flow cell |
|---|---|
| Sequencing Buffer (SB) | 37.5 µl |
| Library Beads (LIB) mixed immediately before use, or Library Solution (LIS), if using | 25.5 µl |
| Recovered DNA library | 12 µl |
| Total | 75 µl |
重要
It is vital that the flow cell priming port and SpotON sample port are closed before removing the waste buffer to prevent air from being drawn across the sensor array area, which would lead to a significant loss of sequencing channels.
Remove the waste buffer, as follows:
- Ensure the priming port and SpotON sample port covers are closed, as indicated in the figure below.
- Insert a P1000 pipette into waste port 1 and remove the waste buffer.
Note: As both the priming port and SpotON sample port are closed, no fluid should leave the sensor array area.
Slide the flow cell priming port cover clockwise to open.
重要
フローセルからバッファーを引き上げる際には注意してください。20~30μl以上は除去せず、ポアのアレイ全体が常にバッファーで覆われていることを確認して下さい。アレイに気泡が入ると、ポアに不可逆的なダメージを与える可能性があります。
プライミングポートを開けた後に、カバーの下に小さな気泡がないかを確認して下さい。気泡を取り除くために少量の液を引き上げます。
- P1000ピペットを200 µ Lに設定して下さい。
- ピペットの先端をプライミングポートに差し込みます。
- 目盛りが220-230 ulと表示されるまでダイヤルを回して、20-30 ulを吸い上げるか、少量のバッファーがピペットの先端に入るのが見えるまでダイヤルを回します。
(注: プライミングポートからセンサーアレイ全体にバッファーがあることを確認してください。
Slowly load 200 µl of the priming mix into the flow cell priming port, as follows:
- Ensure the priming port is open and gently lift open the SpotON sample port.
- Using a P1000 pipette, take 200 µl of the priming mix
- Insert the pipette tip into the priming port, ensuring there are no bubbles in the tip
- Slowly twist the pipette wheel down to load the flow cell (if possible with your pipette) or push down the plunger very slowly, as illustrated in the video above, leaving a small volume of buffer in the pipette tip.
重要
It is vital that the flow cell priming port and SpotON sample port are closed before removing the waste buffer to prevent air from being drawn across the sensor array area, which would lead to a significant loss of sequencing channels.
Remove the waste buffer, as follows:
- Close the priming port and SpotON sample port cover, as indicated in the figure below.
- Insert a P1000 pipette into waste port 1 and remove the waste buffer.
Note: As both the priming port and SpotON sample port are closed, no fluid should leave the sensor array area.
Slide open the priming port cover and gently lift open the SpotON sample port cover.
調製したライブラリーは、ロードする直前にピペッティング混合して下さい。
調製したライブラリー75μlをSpotONサンプルポートからフローセルに滴下します。次の一滴を追加する前に各一滴がポートに入っていることを確認して下さい。
SpotONサンプルポートカバーをゆっくりと元に戻し、バング(カバーの先)がSpotONポートに入ることを確認し、プライミングポートを閉じます。
重要
最適なシークエンス出力を得るために、ライブラリーがロードされたすぐにライトシールドをフローセルに取り付けてください。
ライブラリーがフローセル上にある状態では(ウォッシングやリロードのステップを含める)、フローセルにライトシールドを付けたままにしておくことを推奨します。ライトシールドは、ライブラリーがフローセルから除去された時点で取り外すことができます。
ライトシールドを以下のようにフローセルに設置して下さい。
ライトシールドの先端を慎重にクリップに当てます。 (注: ライトシールドをクリップの下に無理に押し込まないでください。
ライトシールドをフローセルにゆっくりと下ろします。ライトシールドは、フローセルの上部全体を覆うようにSpotONカバーの周囲に取り付けます。
注意
MinIONフローセルライトシールドは、フローセルに固定されていないため、取り付け後の取り扱いには注意が必要です。
最終ステップ
Close the device lid and continue sequencing run on MinKNOW.
ヒント
Library storage recommendations
We recommend storing libraries in Eppendorf DNA LoBind tubes at 4°C for short term storage or repeated use, for example, reloading flow cells between washes. For single use and long-term storage of more than 3 months, we recommend storing libraries at -80°C in Eppendorf DNA LoBind tubes. For further information, please refer to the DNA library stability Know-How document.
5. To store the MinION/GridION Flow Cell for later use
材料
- Flow Cell Wash Kit (EXP-WSH004) or Flow Cell Wash Kit XL (EXP-WSH004-XL)
装置
- P20 pipette and tips
- P1000 pipette and tips
Storage Buffer (S) can be used to flush flow cells for storage for later use or to check number of available nanopores before loading another library.
Thaw one tube of Storage Buffer (S) at room temperature.
Mix contents thoroughly by pipetting and spin down briefly.
Slide the flow cell priming port cover clockwise to open.
After opening the priming port, check for a small air bubble under the cover. Draw back a small volume to remove any bubbles:
- Set a P1000 pipette to 200 µl.
- Insert the tip into the flow cell priming port.
- Turn the wheel until the dial shows 220-230 µl, or until you can see a small volume of buffer/liquid entering the pipette tip.
- Visually check that there is continuous buffer from the flow cell priming port across the sensor array.
Slowly add 500 μl of Storage Buffer (S) through the flow cell priming port.
Close the priming port.
Remove all fluid from the waste channel through waste port 1 using a P1000 pipette.
As both the flow cell priming port and SpotON sample port are closed, no fluid should leave the sensor array area.
重要
It is vital that the flow cell priming port and SpotON sample port are closed before removing the waste buffer to prevent air from being drawn across the sensor array area, which would lead to a significant loss of sequencing channels.
The flow cell can now be stored at 4-8°C.
最終ステップ
When you wish to reuse the flow cell, remove the flow cell from storage, and allow it to warm to room temperature for ~5 minutes.
重要
After performing a flow cell wash or storing your flow cell, we recommend using running a 'Flow cell check' to check number of available nanopores.
Load your flow cell into the device with Storage Buffer (S) and start a Flow cell check to detect the number of active pores. For more information, please visit the Flow cell check section of our MinKNOW protocol.
After the Flow cell check, prime your flow cell and load the library before starting a new sequencing run.
Last updated: 4/25/2024
Document options
