Comparison of Vitrification Effect Before or After In Vitro Maturation
January 31, 2018 updated by: University Hospital, Clermont-Ferrand
Characterization of a Method of Fertility Preservation for Patients Diagnosed for a Cancer
Human oocyte cryopreservation is routinely used for fertility preservation of women who will be exposed to gonadotoxic effect of cancer treatment. After ovarian stimulation, matured oocytes are vitrified. However, this strategy cannot always be used, particularly for hormone-sensitive cancer or when ovarian stimulation is not possible. An approach including immature oocytes and in vitro maturation (IVM) could be considered in these cases. While some qualitative analysis of oocytes vitrified before or after IVM suggest that vitrification should be performed after IVM, little is known about vitrification effects on actin and tubulin cytoskeleton and kinetic of maturation of human ovocytes.
To answer to this question, Investigator performed quantitive analyses comparing matured oocytes from three different groups: vitrified before IVM or after IVM and non-vitrified oocytes. Non-vitrified matured oocytes were used as a control. Different parameters have been analysed during maturation and in matured oocytes.
Study Overview
Status
Status
Unknown
Conditions
Conditions
Intervention / Treatment
Intervention / Treatment
Detailed Description
Immature oocytes were collected from patients (≤37 years old, without endometriosis, Polycystic syndrome or other ovulatory desease) who underwent to ICSI.
In addition, immature oocytes collected from patient diagnosed with cancer will be included in this study.
Oocytes were matured in vitro with IVM medium and vitrified in closed system ("Vitrolife").
Kinetic of maturation were analyzed by Primovision ("Vitrolife") and actin, and spindle organization were studied by microscopy, immunostaining techniques and quantitive analysis.
Study Type
Study Type
Observational
Enrollment (Anticipated)
Enrollment
100
Contacts and Locations
This section provides the contact details for those conducting the study, and information on where this study is being conducted.
Study Locations
-
-
-
Clermont-Ferrand, France, 63003
- Recruiting
- Chu Clermont-Ferrand
-
Sub-Investigator:
- Aïcha METCHAT
-
-
Participation Criteria
Researchers look for people who fit a certain description, called eligibility criteria. Some examples of these criteria are a person's general health condition or prior treatments.
Eligibility Criteria
Eligibility Criteria
Ages Eligible for Study
18 years to 37 years (Adult)
Accepts Healthy Volunteers
Yes
Genders Eligible for Study
Female
Sampling Method
Non-Probability Sample
Study Population
female
Description
Inclusion Criteria:
- - ICSI treatment
- Immature oocytes
- < 37 years old
Exclusion Criteria:
- - Polyckistic Ovarian Syndrome
- Endometriosis
- Ovulatory disease
Study Plan
This section provides details of the study plan, including how the study is designed and what the study is measuring.
How is the study designed?
Design Details
Number of groups / cohorts
3
Cohorts and Interventions
Group / CohortGroup / Cohort |
Intervention / TreatmentIntervention / Treatment |
|---|---|
|
Immature oocytes vitrified before In Vitro Maturation
Immature oocytes were vitrified using closed system vitrification.
After warming, they were cultured during 36 hours in IVM medium and fixed for cellular analysis
|
Immature oocytes were collected from patients (≤37 years old, without endometriosis, Polycystic syndrome or other ovulatory desease) who underwent to ICSI.
In addition, immature oocytes collected from patient diagnosed with cancer will be included in this study.
Oocytes were matured in vitro with IVM medium and vitrified in closed system (Vitrolife).
Kinetic of maturation were analyzed by Primovision (Vitrolife) and actin, and spindle organization were studied by microscopy, immunostaining techniques and quantitive analysis.
|
|
Immature oocytes cultured in vitro before vitrification
Immature oocytes were cultured in vitro in IVM medium during 36 hours.
After IVM, they were vitrified.
After warming, they were fixed for cellular analysis.
|
Immature oocytes were collected from patients (≤37 years old, without endometriosis, Polycystic syndrome or other ovulatory desease) who underwent to ICSI.
In addition, immature oocytes collected from patient diagnosed with cancer will be included in this study.
Oocytes were matured in vitro with IVM medium and vitrified in closed system (Vitrolife).
Kinetic of maturation were analyzed by Primovision (Vitrolife) and actin, and spindle organization were studied by microscopy, immunostaining techniques and quantitive analysis.
|
|
Fresh oocytes
Immature oocytes were cultured in vitro in IVM medium during 36 hours and subsequently, fixed for cellular analysis.
|
Immature oocytes were collected from patients (≤37 years old, without endometriosis, Polycystic syndrome or other ovulatory desease) who underwent to ICSI.
In addition, immature oocytes collected from patient diagnosed with cancer will be included in this study.
Oocytes were matured in vitro with IVM medium and vitrified in closed system (Vitrolife).
Kinetic of maturation were analyzed by Primovision (Vitrolife) and actin, and spindle organization were studied by microscopy, immunostaining techniques and quantitive analysis.
|
What is the study measuring?
Primary Outcome Measures
Primary Outcome Measures
Outcome Measure |
Measure Description |
Time Frame |
|---|---|---|
|
Analysis of maturation kinetic of oocytes vitrified at Prophase-I stage compared to fresh oocytes
Time Frame: at day 1
|
After oocytes retrieval, immature oocytes will be vitrified (Rapid Vit Ovocyte®, Vitrolife) in a closed system (Rapid-I®, Vitrolife) and thawed for in vitro maturation few days after.
The meiotic process will be analyzed by time lapse technology (Primovision®, Vitrolife).
This will permit to score the time of maturation from resumption to polar body extrusion of ovocytes.
|
at day 1
|
Secondary Outcome Measures
Secondary Outcome Measures
Outcome Measure |
Measure Description |
Time Frame |
|---|---|---|
|
Analysis of actin and tubulin cytoskeleton at Metaphase-II stage
Time Frame: at day 1
|
Metaphase-II stage oocytes from both protocols will be used for Immuno-Fluorescence experiments to stain actin, tubulin and chromosomes.
Oocytes will be imaged using confocal microscope to perform high resolution imaging and quantitative image analysis.
The length, position and orientation of the second meiotic spindle will be quantifying.
The actin network and chromosomes will be analyzed quantitatively.
All measurements will be compared with fresh Metaphase-II oocytes used as a control group.
|
at day 1
|
|
Analysis of chromosome segregation during the first meiotic division.
Time Frame: at day 1
|
The first asymmetric division is highly error prone.
To investigate whether chromosomes are segregated accurately after vitrification, we will perform Fluorescence In Situ Hybridization to paint each chromosome after chromosome spread from Metaphase-II stage oocytes from both conditions
|
at day 1
|
|
Analysis of cortical granules distribution in Metaphase-II stage oocytes.
Time Frame: at day 1
|
A staining with Lectin will be used to mark cortical granules of matured oocytes from both protocols to observe whether the vitrification does modify their spatial distribution.
To analyze this staining, we will use quantitative image analysis method.
|
at day 1
|
|
Analysis of maternal factor stabilities.
Time Frame: at day 1
|
Maternal factors stored in the oocyte cytoplasm during oogenesis as proteins and transcripts are essential for the early embryonic development.
To know if the stock of maternal factors is diminished by the vitrification procedure, we will perform Reverse Transcription combined with Real Time PCR to quantify transcript amounts of candidates genes selected from human oocytes databases.
|
at day 1
|
Collaborators and Investigators
This is where you will find people and organizations involved with this study.
Sponsor
Sponsor
Collaborators
Collaborators
Study record dates
These dates track the progress of study record and summary results submissions to ClinicalTrials.gov. Study records and reported results are reviewed by the National Library of Medicine (NLM) to make sure they meet specific quality control standards before being posted on the public website.
Study Major Dates
Study Start (Actual)
Study Start
January 1, 2017
Primary Completion (Actual)
Primary Completion
January 1, 2018
Study Completion (Anticipated)
Study Completion
December 31, 2019
Study Registration Dates
First Submitted
First Submitted
January 24, 2018
First Submitted That Met QC Criteria
First Submitted That Met QC Criteria
January 24, 2018
First Posted (Actual)
First Posted
January 31, 2018
Study Record Updates
Last Update Posted (Actual)
Last Update Posted
February 1, 2018
Last Update Submitted That Met QC Criteria
Last Update Submitted That Met QC Criteria
January 31, 2018
Last Verified
Last Verified
January 1, 2018
More Information
Terms related to this study
Other Study ID Numbers
Other Study ID Numbers
- CHU-372
Drug and device information, study documents
Studies a U.S. FDA-regulated drug product
No
Studies a U.S. FDA-regulated device product
No
This information was retrieved directly from the website clinicaltrials.gov without any changes. If you have any requests to change, remove or update your study details, please contact register@clinicaltrials.gov. As soon as a change is implemented on clinicaltrials.gov, this will be updated automatically on our website as well.
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