Assisted
Hatching or Blastocyst Transfer
MALHOTRA
TEST TUBE BABY CENTRE, AGRA
Introduction
ART
has come to stay. Today there are solutions to all factors of infertility but
still world over the results are not improved to what expected.
Infertility
was conquered in July 1978 by the birth of Louise Brown by the pioneering
efforts of Patrick Steptoe & Robert Edwards. Since 1978 rapid advances have
occurred in the field of assisted reproductive technology. However, live birth
rates have still not reached to our full expections.
The
major factors of success are attributed to poor embryo quality and endometrium.
Even good fertilized embryos show an embryonic block after 4 cell stage to
reach morulla & blastocyst. The embryos which do not have an embryonic
block will ultimately become good blastocysts and hatch and implant.
The
culturing of embryo’s to blastocyst stage will overcome the problem of choosing
which embryo to transfer for the best results. On the other hand older age
group women show implantation failure due to thickened zona and here it has
been proposed to go for assisted hatching techniques by either mechanical,
chemical or laser methods to help in implantation rates.
Various
studies all over the world have shown that blastocyst culturing and transfer
will yield much better pregnancy rates because good-quality blastocysts are
crucial for the development of human embryonic stem cells.
Why Results Not Yet Good
Major Compromising Factors
1.
Poor embryo viability.
2.
Poor endometrial receptivity.
Not So Major
Factors
1.
Lab conditions and equipments.
2.
Media and disposables.
3.
Stimulation and PT. Selection.
4.
Smooth embryo transfer.
Poor Results
·
Low fertilization.
·
Sperms with poor motility.
·
Chromosome anomaly in oocyte and
embryo.
·
Hostile stimulated uterus.
·
A synchronous transfer (Day 2).
·
Reduced viability of embryo cultured in
vitro.
·
Embryo viability questionable on Day 2.
·
Other factors age, stimulation, smooth
transfer, luteal support etc.
Normal
Physiology
·
Oocytes are fertilized
·
Embryo undergo cleavage to compacted or
cavitated stages (Day 4-5).
·
(In fallopian tube)
·
Enters uterus - further cleavage.
·
Dissolution of zona (Day 5).
·
Hatching blastocyst (Day 6)
·
Implantation (Day 7).
Why Blastocyst Culture
?
·
To improve pregnancy and take home baby
rates.
·
Overcome and cell embryonic block.
·
Blastocyst/Uterine synchrony
·
Genetically abnormal embryos will be
weeded out.
·
In vitro blastocyst has a very high TCN
(Total Cell Number) hence better results.
·
PGB and freezing.
·
Development of human embryonic stem
cells though Inner Cell Mass (ICM) by immunosurgery (Future cure of diseases
and genetic therapy).
Choosing Viable Embryo
Selecting
embryos with a high pronuclear (2PN) scores (bongso) and polarity (edwards) and
transferring such embryos after the embryonic block at the 8 cell to blastocyst
stage wil help overcome the problem of choosing the best embryo and most viable
one.
Embryo Assessment
1. Scoring
2. 2 PN embryo quality (Pronucelar score)
3. Cleavage
4. Biochemical/metabolic markers
5. Blastocyst scoring
6. TCN of blastocysts
Other Uses of
Blastocyst
·
Field of ART to improve results.
·
P.G.D.
·
Research
·
Study of early embryogenesis.
·
Study of development of human embryonic
stem cells.
·
Treatment of a variety of genetic and
incurable diseases.
Assisted
Hatching Where and Why ?
·
Women age > 35 yrs.
·
Thick Zona.
·
Before P.G.D.
·
Previously failed implanation.
Assisted
Hatching How ?
·
Mechanical —Zona thinning
—Zona
Drilling
·
Chemical - Acid Tyrode
·
Laser
Advantages of
Blastocyst
·
Viable hardiest embryo for transfer.
·
Weeding genetically defective embryos.
·
Physiological environment.
·
Avoid inheritance of abnormal paternal
genome after ICSI.
·
Non invasive assessment of TCN.
·
Zona free blastocyst by enzymes, better
anchorage of trophoectoderm.
·
Post freeze PN embryos cultured post
thaw.
·
Embryo repair process after ICSI.
·
AID embryo biopsy.
·
AID in assisted hatching.
·
Reduce time of embryo-maternal
dialogue.
·
ICM for development of stem cells.
Culture System
·
Conventional culture media.
·
Human tubal fluid.
·
Co-cultures.
·
Sequentional complex supercompley media
(IVF-to-S2, G 1.2 and G 2.2)
G
1.2TM and G 2.2TM
For a
fertilised egg to develop into a blastocyst in-vitro is an achievement. But
that does not necessarily mean it is viable and will continue to grow. The new
sequential media, G 1.2TM and G 2.2TM have been optimised for blastocysts
development according to the latest research at the Colorado Center for
Reproductive Medicine. Clinical trials have shown up to 50.5% implantation rate
(fetal heart) for blastocysts cultured in G-media*. For more information,
contact IVF Science.
Success
Package
·
PT selection.
·
Proper stimulation (at least 800
cytes).
·
Appropriate blastocyst culture (68-70%
Blastulation rates).
·
Transfer 2/3 blastocysts.
·
Atraumatic transfer (no trauma no
blood).
(Ultrasound
Guided and Mock Previous Transfer)
Success Package
Producing
Quality Oocytes Recovering
Quality Sperms |
Quality Lab Setup
State of the ART Equipments,
Consumables
Timed Oocyte Retrival
Insemination/ICSI
Culture Systems
Blastocyst
Culture
Day
1
Pronuclear
scoring
Growth Media (2 PN) (G 1.2/Medicult)
(Each embryo seperate)
Second
look at non cleaved 25 hrsDay 2
Cleavage
grading (Fragmentation) (Good/Fair/Poor)
G
1.2 Media (48 hrs) Embryo
Transfer (4 cell)
Prepare G 2.2 Dishes (or M3 by medicult)
(Scandinavian)
 |
Day 3
Assess
cleavage
Assisted hatching (8
cell) Transfer to G 2.2 Embryo transfer
Day
4
Assess cleavage culture in G 2.2 (48
hrs)
Blastocyst
culture
Day 4
Priority to highest 20 N score
prepare
one ET dish, one freeze dish & day 6 growth dish (overnight incubate)
Day
5
Blastocyst
assess & scoring
Transfer Freeze Slow growing
Good Spare
2
Blastocysts Blastocysts
(Zona intact) Fresh
G 2.2 media Zona free transfer Day
6
100 µl
droplet of 101 U Pronase Freeze
For 1-11/2 hrs Wash 4 times
Transfer
Zona
free blastocyst
Pregnancy outcomes (Bongso)
Day 3-5 Transfer
Clinical
preg per ET with USG detectable
Cardiac
activity at 7-8 wks 50-57%
Day 2 Transfer
37%
Take
Home Baby Rates
Day
2 15-25%
Day
3 29-42%
Day
4 33%
Day
5 52%
(Singapore Group Bongso ET AL)
Blastocyst Transfer
1. no.
of Patients 39
2. no.
of Embryos for blastulation 53
3. no.
enbryos reached blastocyst 21 (39.62%)
4. no.
of blastocyst transferred 13
5. no.
of ET done 11
6. no.
of clinical pregnancies 3 (27%)
(Fertility Clinic Mumbai) (1998-99)
MTTBC Agra Results (1998-2000)
1. Total cycles 318
2. Day
2 transfers 285 (Pregnancy
23%)
3. Day
3/4 transfer 25 (Pregnancy
28%)
4. Day
5 transfer 8 (Pregnancy
51%)
5. No.
of Embryos for Blastulation is 8 cases = 31
6. Blastulation
sem is 10 embryos
7. No.
of Blastocyst E.T. (cases 2)
Bottom line & take home message
·
Do
assisted hatching at 8 cell stage
·
Micromanipulator
guided blastomere biopsy
·
P.G.D.
·
Culture
to blastocyst
·
Transfer
only P.G.D.—re & blastocyst
·
Overcomes
problem of embryonic block
·
Healthy
embryos (Genetically healthy)
·
Very
good pregnancy rates (> 50%)
·
Very
good take home baby rates (> 40%)
Conclusion
The
techniques of micromanipulator have greatly improved the fertilization rats
upto 90% with Blastocyst culture the pregnancy rate in experted to go upto
40-50%. A very ideal situation for best pregnancy rates would be to make holes
in zona pellucida at the day 3, 8 cell stage by assisted hatching technique by
micromanipulator and doing pre-implantation genetic diagnosis and then
subsequently growing the healthy breached embryos to the blastocyst stage and
then doing a smooth blastocyst transfer on day 5.
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