ANZCTR - Registration

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Trial registered on ANZCTR

Registration number

ACTRN12618001293257

Ethics application status

Approved

Date submitted

27/06/2018

Date registered

31/07/2018

Date last updated

6/03/2020

Date data sharing statement initially provided

6/03/2020

Type of registration

Retrospectively registered

Titles & IDs

Public title

Streamlining lung cancer diagnosis through genomic testing of cytology smears

Scientific title

Streamlining lung cancer diagnosis through genomic testing of cytology smears

Secondary ID [1]

None

Universal Trial Number (UTN)

Trial acronym

DEBUTANT study

Linked study record

Health condition

Health condition(s) or problem(s) studied:

Lung cancer

Tumour genetics

Condition category

Condition code

Cancer

Lung - Non small cell

Respiratory

Other respiratory disorders / diseases

Cancer

Lung - Small cell

Intervention/exposure

Study type

Interventional

Description of intervention(s) / exposure

Patients are those presenting for diagnosis of enlarged mediastinal or hilar lymph nodes where a tissue diagnosis of lung cancer is required by Endobronchial Ulrasound Transbronchial Needle aspiration (EBUS TBNA). Patient study involvement duration is just for the length of time required to take the TBNA samples ( 5-10 minutes) and for the blood test, at time of cannulation ( 1-2 minutes).All cases would have maximum number of 5 passes of the TBNA needle into the node as is usual practice. Main outcome measure is comparing DNA yield from samples taken with differing agitations of the needle within the lymph node. Study question would be whether once in the node there is the same amount of tumour after 3 agitations of the needle versus 10 agitations of the needle, while suction was applied to the needle. this will be measured by DNA content on Rapid-on-site-examination slides ( Diff Quik). All patients would have samples collected with both 3 agitations and 10 agitations measuring the amount of DNA for each of these spearately. Patients would still have a SINGLE cell block sample from ALL needle passes plus a PAP stained slide for conventional histology and immunohistochemistry.

Intervention code [1]

Diagnosis / Prognosis

Comparator / control treatment

the comparison is between 3 agitations of the TBNA needle and 10 agitations of the needle on alternating passes into the lymph node. There is no control group. All patients will be having the procedure with the objective of diagnosing lung cancer, and there is NIL impact on any treatment decision based on this question. the molecular analysis of the cell block is still the mechanism by which molecular treatment decisions will be made and this is not affected by the analysis of these ROSE slides.

Control group

Uncontrolled

Outcomes

Primary outcome [1]

DNA content of slides of ROSE slides from EBUS TBNA NEEDLE passes made with 3 agitations of the needle within the node versus slides made with 10 agitations. DNA quantitation ( ng per slide) will be the main outcome measure along with tumour smear cellularity on the ROSE slides. Genomic DNA will be extracted from the entirety of DQ cytology slides using a QIAamp DNA Micro Kit (QIAGEN Inc., Germantown, MD). DNA yields will be measured using a Qubit™ dsDNA BR Assay (Thermo Fisher Scientific, Inc.Waltham, MA).

Timepoint [1]

there is only one timepoint in the study ie at the time of diagnosis- all samples processed at that time. Is not a followup study

Primary outcome [2]

A different endpoint is to examine which parts of the sample have the most DNA as they are extruded back out of the needle- the first drops out, or the last drops. DNA content of ROSE slides made by comparing the first drops of sample ( to come out of the needle after withdrawal from the patient) versus the last drops of sample ( to come out of the needle after withdrawal from the patient. Measured as ng DNA

Timepoint [2]

There is only one timepoint in the study ie at the time of diagnosis- all samples processed at that time. Is not a followup study.

Secondary outcome [1]

In a full exploration of Next generation sequencing on these samples , DNA in liquid based cytology media ( including methanol as well as RNA Later) will be analysed for whole exome and whole genome sequencing. the success of these samples will be compared to the original diff quik slides as a way of predicting tumour DNA content in the Liquid based cytology media.

Timepoint [1]

There is only one timepoint in the study ie at the time of diagnosis- all samples processed at that time. Is not a followup study.

Eligibility

Key inclusion criteria

Patients with enlarged mediastinal and/ or hilar lymph nodes suggestive of lung cancer requiring EBUS TBNA for tissue diagnosis.

Minimum age

40 Years

Maximum age

No limit

Sex

Both males and females

Can healthy volunteers participate?

Key exclusion criteria

Patients deemed not suitable for bronchoscopy by their treating clinician
Patients deemed unfit for bronchoscopy on the basis of
• Severe respiratory insufficiency or hypoxia, moderate-to-severe hypoxemia or any degree of hypercarbia
• Continuous use of anticoagulants (eg, heparin, warfarin) ADP-Receptor inhibitors (Clopidogrel), GP-IIB/IIIA- inhibitors (Abciximac), fish oil, etc) which cannot be discontinued.
• Uncorrectable coagulopathy or bleeding diathesis
• Platelet dysfunction or platelet count <100×10
• History of major bleeding with bronchoscopy
• Partial tracheal obstruction or obstruction of the superior vena cava
Any other severe or life-threatening comorbidity that could increase the risk of bronchoscopic biopsy

Study design

Purpose of the study

Diagnosis

Allocation to intervention

Non-randomised trial

Procedure for enrolling a subject and allocating the treatment (allocation concealment procedures)

Methods used to generate the sequence in which subjects will be randomised (sequence generation)

We will use a pre printed random order for which needle pass is done first ( whether it be 3 agitations or 10 agitation)

Masking / blinding

Who is / are masked / blinded?

Intervention assignment

Parallel

Other design features

2 ebus tbna needles will be used- one for 3 agitations, one for 10 agitations

Phase

Not Applicable

Type of endpoint/s

Bio-equivalence

Statistical methods / analysis

For a non inferiority study of 3 agitations versus 10 agitations we need 134 patients; outcome measure is DNA yield. A clinically meaningful difference (as shown from our pilot study) was taken as 1000ng, and the standard deviation from our study DNA yield of cytology slides was 1970 ng.
If there is truly no difference between the standard and experimental sampling method, then 134 patients are required to be 90% sure that the lower limit of a one-sided 95% confidence interval (or equivalently a 90% two-sided confidence interval) will be above the non-inferiority limit of -1000. Hence we would study 140 patients

Recruitment

Recruitment status

Recruiting

Date of first participant enrolment

Anticipated

Actual

31/05/2018

Date of last participant enrolment

Anticipated

1/03/2022

Actual

Date of last data collection

Anticipated

1/03/2022

Actual

Sample size

Target

140

Accrual to date

120

Final

Recruitment in Australia

Recruitment state(s)

NSW,QLD,SA,VIC

Recruitment hospital [1]

Gold Coast University Hospital - Southport

Recruitment hospital [2]

Sunshine Coast University Private Hospital - Birtinya

Recruitment hospital [3]

Liverpool Hospital - Liverpool

Recruitment hospital [4]

Royal Melbourne Hospital - City campus - Parkville

Recruitment hospital [5]

The Royal Adelaide Hospital - Adelaide

Recruitment postcode(s) [1]

4029 - Royal Brisbane Hospital

Recruitment postcode(s) [2]

4215 - Southport

Recruitment postcode(s) [3]

4575 - Birtinya

Recruitment postcode(s) [4]

2170 - Liverpool

Recruitment postcode(s) [5]

3050 - Parkville

Recruitment postcode(s) [6]

5000 - Adelaide

Funding & Sponsors

Funding source category [1]

Commercial sector/Industry

Name [1]

Olympus Australia

Address [1]

3 Acacia Place, Notting Hill, VIC 3168, Australia

Country [1]

Australia

Primary sponsor type

Hospital

Name

Royal Brisbane and Womens Hospital

Address

Block 7 Royal Brisbane and Womens Hospital Butterfield Street Herston Qld 4029

Country

Australia

Secondary sponsor category [1]

Charities/Societies/Foundations

Name [1]

Cancer Council of Queensland

Address [1]

553 Gregory Terrace
Fortitude Valley QLD 4006

Country [1]

Australia

Secondary sponsor category [2]

Charities/Societies/Foundations

Name [2]

Cancer Australia

Address [2]

PO Box 1201, DICKSON ACT 2602

Country [2]

Australia

Ethics approval

Ethics application status

Approved

Ethics committee name [1]

Royal Brisbane and Womens Hospital Human Research Ethics Committee'

Ethics committee address [1]

Block 7 Royal Brisbane and Womens Hospital Butterfield Street Herston Qld 4029

Ethics committee country [1]

Australia

Date submitted for ethics approval [1]

29/05/2017

Approval date [1]

21/09/2017

Ethics approval number [1]

HREC/17/QRBW301

Summary

Brief summary

 The purpose of this study is to assess whether a new screening method is effective in providing a clearer picture of lung cancer.

Who is it for?
You may be eligible for this study if you are about to undergo endobronchial ultrasound guided transbronchial needle aspirate (EBUS-TBNA) in order to assess the presence of lung cancer. 

Study details
There are 2 samples which will be used from patients- one is samples from the  EBUS TBNA test and the other is a blood test.  The EBUS TBNA test will still have the goal of making the diagnosis your doctor is aiming to obtain. This sample will also be used for determining the best way this needle test should be done and how the maximum information about the genes in a cancer can be obtained form this test.  Very importantly this new method should significantly improve the samples to make them ideal for very rapid analysis to obtain the information about the all-important genes. 
We have done studies to use lung samples to simultaneously test 48 genes with one machine. We want to take this further in 2 ways- one is to streamline the best way of actually drawing out the tiny amounts of material from the node. For example we will compare moving the needle within the nodes 3 versus 10 times. The other is to send the sample to a different machine which can sample the entire range of genes in the cancer- not just 48. We want to see if this is possible to do with the tiny amounts of sample we will send to the machine - only a drop or 2 of node sample.
The blood test will be used to compare your normal genes with gens of any cancer in the sample. This blood test will be taken at the time your cannula is placed and will not hurt.

 It is hoped that this research will help determine whether this testing provides a better picture of lung cancer to patients and thus further helps doctors determine how best to treat it.

Trial website

Trial related presentations / publications

Public notes

Attachments [1]

/AnzctrAttachments/375444(v27-06-2018-13-30-22)-Final Fielding Next Gen protocol version 3.doc (Protocol)

Attachments [2]

/AnzctrAttachments/375444-fieldingd_ETHICS APPROVAL.pdf (Ethics approval)

Attachments [3]

/AnzctrAttachments/375444-picf_non-interventional_self_fielding MASTER RBWH FINAL.doc (Participant information/consent)

Attachments [4]

/AnzctrAttachments/375444-rccm Fielding et al.pdf (Publication)

Contacts

Principal investigator

Name

A/Prof David Fielding

Address

Dept Thoracic Medicine James Mayne Building Royal Brisbane and Womens Hospital Butterfield Street Herston Qld 4029

Country

Australia

Phone

+61736464241

Fax

+61736465651

[email protected]

Contact person for public queries

Name

David Fielding

Address

Dept Thoracic Medicine James Mayne Building Royal Brisbane and Womens Hospital Butterfield Street Herston Qld 4029

Country

Australia

Phone

+61736464241

Fax

+61736465651

[email protected]

Contact person for scientific queries

Name

David Fielding

Address

Dept Thoracic Medicine James Mayne Building Royal Brisbane and Womens Hospital Butterfield Street Herston Qld 4029

Country

Australia

Phone

+61736464241

Fax

+61736465651

[email protected]

Data sharing statement

Will individual participant data (IPD) for this trial be available (including data dictionaries)?

No/undecided IPD sharing reason/comment

What supporting documents are/will be available?

Doc. No.	Type	Attachment
7267	Study protocol	375444-(Uploaded-18-02-2020-17-41-09)-Study-related document.doc
7268	Informed consent form	375444-(Uploaded-18-02-2020-17-42-44)-Study-related document.doc
7269	Ethical approval	375444-(Uploaded-18-02-2020-17-43-25)-Study-related document.pdf

Results publications and other study-related documents

Documents added manually

No documents have been uploaded by study researchers.

Documents added automatically

No additional documents have been identified.

Trial Review

Documents added manually

Documents added automatically