ANZCTR - Registration

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Trial registered on ANZCTR

Registration number

ACTRN12612000422820

Ethics application status

Approved

Date submitted

11/04/2012

Date registered

16/04/2012

Date last updated

16/04/2012

Type of registration

Prospectively registered

Titles & IDs

Public title

A randomised study of IVF patients to assess whether freezing all of the embryos and transferring them in a later natural, unstimulated cycle results in a higher pregnancy rate than transferring an embryo 5 days after egg collection

Scientific title

A Randomised Controlled Trial to determine the effect of Elective Embryo Cryopreservation and Subsequent Transfer in a Natural Menstrual Cycle on clinical pregnancy rates in infertile females.

Secondary ID [1]

nil

Universal Trial Number (UTN)

Trial acronym

Linked study record

Health condition

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

Infertility

Condition category

Condition code

Reproductive Health and Childbirth

Fertility including in vitro fertilisation

Intervention/exposure

Study type

Interventional

Description of intervention(s) / exposure

Both study groups will undertake a stimulated IVF cycle.
The first( intervention) group will have all embryos cryostored electively for transfer in a later natural menstrual cycle.
The second group will have the best quality embryo transferred to the endometrial cavity fresh and all remaining embryos cryostored.
The protocol for the second group is standard practice today.
Both groups undertake the same drug regime therefore there is no difference in drug intervention

Intervention code [1]

Treatment: Other

Comparator / control treatment

All cycles will be using a standard antagonist protocol - Day 1 FSH <12, Oestrogen < 200pmol/L

Commence FSH stimulation on day 2 of cycle with rFSH (Puregon, Organon) 150 Units +/- 50 Units per day (dose decided by physician based on BMI and age)

Fixed daily dose of Orgalutran 0.25micrograms subcutaneous injection per day commenced on day 5 of stimulation

Estradiol levels will be measured on Day 3/4 and Oestradiol, Progesterone, LH level and follicle measurements on day 8 and 10 of stimulation

FSH and Orgalutran injections continued until there are 2 or more lead follicles greater than 17mm in diameter. On that day Ovidrel Serono 250 micrograms subcutaneous injection will be used to trigger ovulation

Trans-vaginal oocyte collection thirty-six hours after trigger injection under local anaesthetic and sedation or General anaesthetic.

IVF or ICSI in the laboratory as per Genea laboratory protocol

There must be at minimum 2 embryos for cryostorage at 9:00 am on day 5.
One blastocyst will be transferred in the fresh embryo group and vitrification of all other suitable embryos.

All embryos will be vitrified in the elective freezing group.
Luteal phase support with Pregnyl 1500 U subcutaneous injection on day two and six post OPU or Cinone 8% vaginal suppository if judged to be at higher risk of hyper-stimulation syndrome.

All frozen embryo transfers will be in a natural cryo cycle with transfer of a single thawed embryo on
ovulation day +5. Ovulation will be determined by LH surge > 20 IU Endometrial thickness must be >6mm.

The whole cycle will last approximately 28 days

Control group

Active

Outcomes

Primary outcome [1]

The primary endpoint is the clinical pregnancy rate in each group, defined as a fetal heartbeat seen on ultrasound at 7 weeks.

Timepoint [1]

Outcome is assessed by transvaginal ultrasound at 7 weeks.

Secondary outcome [1]

The number of good-quality embryos by assessment of morphology by embryologist

Timepoint [1]

At completion of study

Secondary outcome [2]

Proportion of subjects in each group that had 2 or more embryos suitable for vitrification

Timepoint [2]

At completion of study

Secondary outcome [3]

Cumulative clinical pregnancy rates

Timepoint [3]

At completion of study

Secondary outcome [4]

Implantation rate assessed by positive beta hCG serology on day of pregnancy test.

Clinical miscarriage rate assessed by finding of an intrauterine sac on transvaginal ultrasound but no resulting on going pregnancy

Timepoint [4]

At completion of study

Secondary outcome [5]

Live birth rates

Timepoint [5]

2 years following completion of study

Secondary outcome [6]

Perinatal complications of placentation

Timepoint [6]

2 years following completion of study

Secondary outcome [7]

Blastulation anomalies

Timepoint [7]

2 years following completion of study

Eligibility

Key inclusion criteria

Females of infertile couples for whom controlled ovarian stimulation and IVF with or without ICSI is indicated
Age at least 20 years but not more than 38 years at the time of screening
Regular menstrual cycles with a range of 24-33 days
BMI 18-28
AMH 5-20

Minimum age

20 Years

Maximum age

38 Years

Sex

Females

Can healthy volunteers participate?

Key exclusion criteria

Previous IVF treatment cycle that resulted in <6 follicles on Day 8 ultrasound
More than 2 previous unsuccessful stimulated cycles
History of/or current endocrine abnormality such as polycystic ovary syndrome or evidence of ovarian dysfunction
Any clinically significant abnormal laboratory value (TSH, PRL, SHBG, Test)
Any ovarian and/or abdominal abnormality that would interfere with adequate ultrasound investigation of at least one ovary
Only one ovary
Contra-indications for the use of gonadotrophins
Alcohol or drug abuse, or history thereof, within the 12 months preceding signing informed consent
Smokers

Study design

Purpose of the study

Treatment

Allocation to intervention

Randomised controlled trial

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

Randomisation will occur at the time of nurse interview by opening an opaque envelope and allocating the patient to one of the 2 treatment groups. The 1st group will have the best embryo transferred in that cycle and all others frozen.
the 2nd group will have all embryos frozen and transferred in a natural frozen cycle at a later date

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

Simple randomisation using sealed opaque envelope and allocating
the patient to one of the 2 treatment groups dependant on the content of the envelope.
There will be 100 envelopes allocating the patient to treatment in each group

Masking / blinding

Open (masking not used)

Who is / are masked / blinded?

Intervention assignment

Parallel

Other design features

Phase

Not Applicable

Type of endpoint/s

Efficacy

Statistical methods / analysis

Recruitment

Recruitment status

Not yet recruiting

Date of first participant enrolment

Anticipated

1/05/2012

Actual

Date of last participant enrolment

Anticipated

Actual

Date of last data collection

Anticipated

Actual

Sample size

Target

200

Accrual to date

Final

Recruitment in Australia

Recruitment state(s)

Funding & Sponsors

Funding source category [1]

Self funded/Unfunded

Name [1]

Address [1]

Country [1]

Australia

Primary sponsor type

Individual

Name

Mark Livingstone

Address

Level 3,
23 - 25 O'Connell Street,
Sydney
NSW 2000

Country

Australia

Secondary sponsor category [1]

Commercial sector/Industry

Name [1]

Genea

Address [1]

321 Kent Street,
Sydney,
NSW 2000

Country [1]

Australia

Other collaborator category [1]

Individual

Name [1]

Steven MacArthur

Address [1]

321 Kent Street,
Sydney,
NSW 2000

Country [1]

Australia

Ethics approval

Ethics application status

Approved

Ethics committee name [1]

Genea ethics committee

Ethics committee address [1]

321 Kent Street,
Sydney,
NSW 2010

Ethics committee country [1]

Australia

Date submitted for ethics approval [1]

Approval date [1]

23/03/2012

Ethics approval number [1]

Summary

Brief summary

At Genea frozen embryo transfer pregnancy success rates have improved to a level close to fresh embryo transfer success rates.  The embryos used in the frozen cycles are the second and third best embryos - as graded for development rate and morphology- compared to the embryos transferred in the fresh cycles when the best quality embryo is selected for transfer to the uterus.  The hormone stimulation undertaken prior to oocyte collection may affect the endometrium (uterine lining) - advancing it to a stage whereby the embryo implantation prospect could be  impaired  and therefore reducing the chance of an ongoing pregnancy.  The hypothesis is that freezing of all embryos may help to overcome any reduction in implantation potential by allowing improved synchronisation between the embryo and the endometrium, leading to both higher implantation and pregnancy rates.


There are a number of causes of pregnancy failure following IVF treatment including genetically abnormal embryos, poor quality embryos and potentially a non-receptive uterine environment.  The transfer of genetically and morphologically normal embryos into a non-receptive uterine environment will likely not achieve a pregnancy.  Generally the suitability of the uterine environment is measured by ultrasound.  However such measurement is not able to provide full information on how the uterus has developed under the influence of hormone stimulation drugs used routinely in an IVF treatment cycle.

Genea has extensive experience with vitrification technology having been the first clinic to introduce the procedure into routine clinical practise in Australia, January 2006.  Subsequently the technology has been performed routinely in all Genea laboratories following IVF, ICSI and PGD treatment cycles.  More than 1000 babies have now been born after vitrification at Genea.  

The vitrification procedure used in this study will be applied to embryos cultured at the Genea Kent Street laboratory for 5 days (blastocyst stage).   

By vitrifying and NOT TRANSFERRING embryos in “routine” IVF cycle fresh, we wish to see if this will:
increase the chance of fetal heart pregnancy and increase the chance of a live born baby

Trial website

Trial related presentations / publications

Public notes

Contacts

Principal investigator

Name

Address

Country

Phone

Fax

Contact person for public queries

Name

Mark Livingstone

Address

23-25 O'Connell Street
Sydney
NSW 2000

Country

Australia

Phone

+61407325720

Fax

+61292323416

[email protected]

Contact person for scientific queries

Name

Mark Livingstone

Address

23-25 O'Connell Street
Sydney
NSW 2000

Country

Australia

Phone

+61407325720

Fax

+61292323416

[email protected]

No information has been provided regarding IPD availability

What supporting documents are/will be available?

No Supporting Document Provided

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