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SCREENING WHAT TESTS WHEN &
WHAT NEXT?
NARENDRA MALHOTRA
JAIDEEP MALHOTRA
RISHABH BORA
NEHARIKA BORA
KANIKA BANSAL
MANJEET MEHTA
Global rainbow health care India
Reference Material
• New WHO guidelines on antenatal care –
Systematic review BJOG 2016;123:519-28
• Guidelines by Government of western Australia
• SOGC guideline on Prenatal Screening
• RCOG / NICE Guidelines
• FOGSI expert group(TOG)
“I get by with a little help from my friends”
Dr S Suresh
Dr Ashok Khurana
Dr Pratima Radhakrishnan
Dr Deepika Deka
Dr Anita Kaul
Dr Feroza Begum
THANK YOU FRIENDS FOR HELPING
AND CONTRIBUTING TO THIS
SCREENING PRINCIPLES
Screening is done for:
• Disorders with common prevalence
• Have significant impact on perinatal
mortality & morbidity
Conditions to be fulfilled:
• Accessibility, Availability , Affordability
• Must understand Cost of burden of the disease vs
cost of screening
What Do Screening Tests Do?
1. Identify patients “at risk” for a disorder in an
“unsuspected” population
2. “Filters” patients for further diagnostic testing
3. Results are given as “high risk” or “low
risk” based on a “cut off” value
PRENATAL SCREENING
• I TRIMESTER
• History, MAP,
Ut A doppler /
Biochem
• II TRIMESTER(?)
• UT A doppler
• CERVICAL
LENGTH – II
trimester
• I & II
TRIMESTERS
• ULTRASOUND
• BIOCHEMISTRY
• CELL FREE DNA
• I & II TRIMESTERS
ANEUPLOIDY ANOMALY
PRE-
ECLAMPSIA
PRETERM
BIRTH
PRENATAL TESTING
SCREENING TEST
•Provides individual risk assessment
•Advantages
• Lowers the number of procedures done for diagnosis
• Lowers the procedure related complications
•Disadvantages
• Non diagnostic
• May miss target
DIAGNOSTIC TEST
•A test that WILL identify a disease or defect
•Advantages
• Definitive
•Disadvantages
• Risk associated with diagnostic procedure/s
Magnitude of Problem
Congenital & Genetic Disorders in India
Disorder Frequency
at birth in stillbirths in NN Deaths
Congenital 2-5% (1:50 , 6 lacs/yr) 13.6 % 7 – 10 %
Malformations
Chromosomal 0.5% ( DS – 1:916 , 22,000 / yr )
Single Gene 0.6% ( B- thal – 1:2700 , 9000/ yr ; SCD - 5,200 /yr ;
DMD + SMA - 4,500 / yr )
( IC Verma , Preventive Genetics ,2006 )
Chromosomal defects
Source:
Kagan KO et al. Screening for Chromosomal Abnormalities by First Trimester Combined Screening and Noninvasive Prenatal Testing. Ultraschall in Med 2015; 36:40-46)
FOGSI OLD CHECK LIST OF 2009,MODIFIED IN 2017 AT FOGSI T.O.G.
SCREENING FOR ANEUPLOIDY
• Trisomy 21 - Down syndrome - 1 in 800
• Trisomy 18 – Edwards synd. - 1 in 10,000
• Trisomy 13 – Patau’s syndrome > 1 in 10,000
Apriori Risk
MATERNAL AGE,
Previous screening)
Identify
markers
(USG, Biochem)
Modify Risk
Identify
Patients for
invasive testing
12
TEST FIRST TRIMESTER SECOND TRIMESTER
CRL 45-84 BPD 30mm -51mm
10 11 12 13 14 15 16 17 18 19 20
Sequential Screen
NT,
PAPP-A, hCG
+PLGF
AFP, hCG, uE3,
Inhibin A
CONTINGENT
SCREEN
NB/ DV/TR
Serum Integrated
Screen
hCG , PAPP-A AFP, hCG, uE3,
Inhibin A
Quad Screen
E-FTS
PAPP-A, hCG
+AFP +PLGF
AFP, hCG, uE3,
Inhibin A
1
4
w
G
r
a
y
Z
o
n
e
THE TIMELINES FOR SCREENING
NIPS – after 10 weeks – ideal before 17 weeks to help decision making < 20 weeks
First trimester screening FOR CHROMOSOMAL ANOMALIES
FETAL
CROWN
FETAL
RUMP
NT/NB
DV
TR
First Trimester Screening – The yield
Test Name
Time of
Test(in
Weeks)
Markers
DR(%) FPRs ( % )
Early Biochemistry 9-10^+6 MA+hCGB, PAPP-A
~60-65 5 %
COMBINED FIRST
TRIMESTER
SCREENING
11-13^+6 MA+hCGB, PAPP-A+NT
~90-91 3 %
11-13^+6 MA+hCGB, PAPPA+NT
+NB+tri cuspid flow+facial
angle+Ductus Venoses
~95% 3 %
Penta Screening 10-
13^+6
MA+ hCGB, PAPPA, PIGF,
DIA+NT+NB
98 % 1.2 %
BE HAPPY TEST
JOGI – Feb 2019
Objective
• To derive a risk calculation algorithm suitable for
use in India when screening for Down’s
• Syndrome using four first-trimester maternal
serum markers either alone or with ultrasound
nuchal translucency (NT).
Enhanced Combined test
1: 250 cutoff Enhanced
Combined
EFTS
COMBINED TEST
DETECTION RATE 90% 85%
FALSE +ve rate 1.4% 1.8%
Screening for Trisomy 21 at 11- 14 weeks
2-stage (contingency) screening- UK system
COMNINED TEST (NT+BIOCHEM) FOR ALL
Fetal NT and
free BhCG and
PAPP-A at 12 wks
High risk
>1:250
low risk
<1:1000
CVS
Reassure
Borderline risk
1 in 251-1:1000
Further
screening
Nasal bone
DV, TR
NIPS
99
First Trimester
Second Trimester
Third Trimester
Second Trimester Screening
Screening
Strategy
Time of
Test(in
Weeks)
Markers Used DR(%) FPRs ( %)
Triple Test 15-21^+6 MA+AFP,hCGB, uE3 ~65-70 5-7%
Quadruple
Test
15-21^+6 MA+AFP,hCGB, uE3
,Inhibin-A
~70-75 5-7%
Integrated
Test
15-21^+6 1st Trimester – PAPP-A
11-13+6/7weeks
(11 Wks is Ideal)
2nd Trimester –Quad
AFP, uE3, FBhCG,
Inhibin-A
(15-17 Wks is ideal)
93% 3 %
Contingent II trimester “Genetic sonogram”
To modify risks after
FTS combined,
Quadruple
Or
Integrated screening
Needs high USG expertise
Software for calculation
ARSA Absent NB
When there are major structural defects
NO screening is offered – Direct testing is preferred
SCREENING FOR FETAL ANOMALIES- I TRIMESTER
70% detection rate if a systematic scan is done
Pre-Eclampsia
• Adaptive disease when there is relative
placental imbalance (Utero Placental
mismatch)
– Late onset may be beneficial to the baby –
improved quality of survival in late mild PE
• Early onset may have implications for mother /
baby
SCREENING FOR PE
• Maternal history
• Maternal blood pressure
• Uterine artery doppler
• Biochemical markers
• Combination ..
PAPP-A / PLGF
First trimester screening for Preeclampsia
Maternal serum PIGF,
Mean arterial Blood pressure
- Implantation
- Maternal artery remodelling
Detection rate – 90%
0
10
20
30
Falsepositive(%)
Doppler
12%
30%
PP13
9%
Doppler
& PP13
History + MAP + UT A doppler + PLGF & PAPP-A
• 93% detection rate (5% FPR) for early
preeclampsia (<34 weeks)
Poon LC et al Hypertension 2009
A combination of markers at 11-
13 weeks is ideal
• Low-dose aspirin initiated in early pregnancy is an
efficient method of reducing the incidence of
preeclampsia and IUGR.
(Obstet Gynecol 2010;116:402–14)
Is there intervention??
Is there intervention if screened in first trimester?
• Low-dose ASA may prevent as many as 50% of
cases of PE & IUGR when treatment is initiated
before 16 weeks of gestation
Bujold E, et al Obstet Gynecol 2010;116(2 Pt 1):402–14.
Bujold E et al J Obstet Gynaecol Can 2009;31:818–26.
DIAGNOSTIC TESTS
AFTER SCREENING
WHAT TO ORDER
AND
WHAT TESTS TELLS WHAT
DIAGNOSTIC CONFIRMATORY TESTING AFTER SCREEN POSITIVE
RESULT
• What tests:
–Karyotyping
• Aneuplodies , structural rearrangements
–Microdeletions
• 22q most common
–Microarray
• Increased NT – Normal Karyotype
• Deletions & duplications
1. Karyotyping
2. Fluorescence In Situ Hybridization (FISH)
3. Polymerase Chain Reaction (PCR)
4. Array‐based comparative genomic
hybridization (array CGH) i.e. chromosomal
microarray analysis (CMA) ,next-generation
sequencing (NGS) , whole-exome sequencing
Shaffer LG, Bui T‐H. 2007. Molecular cytogenetic and rapid aneuploidy detection methods in
prenatal diagnosis. Am J Med Genet Part C Semin Med Genet 145C:87–98.
Testing with foetal cells
Karyotype can detect
• Some specific abnormalities e.g.
- Trisomies (21,18,13), Klinefelter's syndrome
(XXY and other variations), Triple X syndrome
(XXX)
- Monosomy : Turner syndrome (X0)
• Some Chromosomal deletions
- Cri-du-Chat syndrome (missingCh5)
- Williams syndrome (missing Ch7)
• Translocations : Robertsonian translocations
Limitation : Cannot detect specific gene mutations e.g. cystic fibrosis ,
Thalassemia. Resolution limited to around 5 Mb.
Molecular cytogenetics :FISH
(Florescence In Situ Hybridization)
• Is a cytogenetic technique used to detect and localize
the presence or absence of specific DNA sequences on
chromosomes
• Allows visualization of small region on chromosome too
small to be identified by karyotyping(submicroscopic
deletion)
• Unlike Karyotype(21days) results available with in 24
to 72 hrs as done on interphase nuclei
QF-PCR
 has recently entered the field of prenatal diagnosis to
overcome the need to culture fetal cells, allow rapid
diagnosis of some selected chromosomal anomalies.
 has the advantage of being much less expensive and
allowing the simultaneous processing of much larger
number of samples than FISH.
 Can detect mosaicism of about 20–30% and is superior
to both traditional karyotyping and interphase FISH
for the identification of maternal cell contamination
[ Donaghue et al., 2005]
QF-PCR: Offerings
QF-PCR BASIC QF-PCR EXTENDED
Coverage • Trisomies :13,18,21
and Gonsomal
Aneuploidies
 Trisomies :13, 18,21, 15,16,22,
Gonosomal Aneuploidies
 20 common microdeletions and
microduplications:
 DiGeorge Syndrome,Langer-
Giedons Syndrome,Smith-
Magnenis Syndrome,Miller-
Dieker Syndrome,Williams-
Beuren Syndrome,Potoscki-
Lupuski Syndrome
Microarray Analysis
Can identify chromosomal aneuploidy , large structure
changes as well as submicroscopic abnormalities that
are too small to be detected by traditional modalities
A DNA microarray is a thin-sized chip that has been
spotted at fixed locations with thousands of single-
stranded DNA fragments corresponding to various genes
of interest
A single microarray may contain 10,000 or more spots,
each containing pieces of DNA from a different gene
Introduction of chromosomal microarray
analysis into prenatal diagnosis
• CMA is now the first-tier genetic diagnostic test for
children and adults with multiple congenital anomalies,
genetic syndromes, and intellectual and developmental
disabilities, diagnostic yield - 15 to 20%
• CMA is recommended as a primary test, by ACOG ,after
USG finding of structural abnormality unless the
abnormality is “strongly suggestive” of a particular
aneuploidy
• CMA suitable for analysis of stillbirth samples & early
miscarriages , it does not require actively dividing cells
Miller DT, Adam MP, Aradhya S, et al. Am J Hum Genet. 2010;86(5):749–64. Hillman SC, McMullan DJ, Hall G, et al. :
Ultrasound Obstet Gynecol. 2013;41(6) ACOG Practice Bulletin,163:2016
Next Generation Sequencing(NGS)
• Sequence each of the 3 billion bases in the human
genome multiple times providing an insight into
unexpected DNA variation missed by other methods.
• Can sequence entire genomes or specific areas of
interest, including all 22 000 coding genes (a whole
exome) or small numbers of individual genes
• By providing a base-by-base view of the genome, NGS
can identify single nucleotide variants (SNV), small
structural changes, and balanced translocations
• increasing information while decreasing costs with a
genome-wide view of variation.
Arch Dis Child Educ Pract Ed. 2013 Dec; 98(6): 236–238
SEQUENCING
KARYOTYPE NEXT GENERATION
SEQUENCING
MICROARRAY
Whole-exome sequencing(WES)
• Congenital abnormalities identified USG , karyotype and
CMA reveal a diagnosis in up to 20–30%, for the
remainder, single-gene tests or gene panels, may be
useful
• CMA and NGS based methods, such as targeted gene-
panel sequencing and, recently, whole-exome
sequencing (WES), has enabled to diagnose more fetal
genetic conditions
• In WES, majority of coding exons, which represent only
2% of the genome but contain 85% of disease-causing
mutations, are sequenced
Lee H, Deignan JL, Dorrani N, et al. : . JAMA. 2014;312(18). Gilissen C, Hehir-Kwa JY, Thung DT, et al. : Nature.
2014;511(7509) Beaulieu CL, Majewski J, Schwartzentruber J, et al. : . Am J Hum Genet. 2014;94(6)
Cont--
• The American College of Medical Genetics and
Genomics recommends considering WES when
specific genetic tests available for a phenotype,
including targeted sequencing , have failed to
determine a diagnosis in a fetus with multiple
congenital anomalies suggestive of a genetic
disorder
• Routine use of whole-genome or whole-exome
sequencing is not recommended outside of the
context of clinical trials
ACMG Board of Directors. Genet Med 2012;14:759–61 , ACOG Practice bulletin ,Number 682, December 2016
Take home message
SCREEING SHOULD BE OFFERED TO ALL
POPULATION IRRECPECTIVE OF RISK
While
• Testing should be focused on the individual
patient's risks, reproductive goals, and preferences
Patients should understand the benefits and
limitations , including the conditions that will not be
detected by tests
PRE AND POST TEST COUNCELLING IS VERY
IMPORTANT
Various Integrated screening in
strategies (1st and 2nd trim)
Main strategies:
• Fully Integrated
• Step-wise sequential
• Contingent screening
1st trimester:
NT, PAPP-A
No risk estimate
2nd trimester:
Fb-hCG, AFP, uE3, (± Inhibin)
Final risk estimate:
All markers
1st trimester:
NT, PAPP-A, Fb-hCG
Risk estimate
Final risk estimate:
All markers
CVS
NIPT
High risk
Low risk
2nd trimester:
Fb-hCG, AFP, uE3, (± Inhibin)
1st trimester:
NT, PAPP-A, Fb-hCG
Risk estimate
2nd trimester:
Fb-hCG, AFP, uE3, (± Inhibin)
Final risk estimate:
All markers
CVS
NIPT
HR
Borderline risk
No further
screening
LR
Thank you
Screen with the right test at the right time

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SCREENING WHAT TESTS WHEN & WHAT NEXT?

  • 1. SCREENING WHAT TESTS WHEN & WHAT NEXT? NARENDRA MALHOTRA JAIDEEP MALHOTRA RISHABH BORA NEHARIKA BORA KANIKA BANSAL MANJEET MEHTA Global rainbow health care India
  • 2. Reference Material • New WHO guidelines on antenatal care – Systematic review BJOG 2016;123:519-28 • Guidelines by Government of western Australia • SOGC guideline on Prenatal Screening • RCOG / NICE Guidelines • FOGSI expert group(TOG)
  • 3. “I get by with a little help from my friends” Dr S Suresh Dr Ashok Khurana Dr Pratima Radhakrishnan Dr Deepika Deka Dr Anita Kaul Dr Feroza Begum THANK YOU FRIENDS FOR HELPING AND CONTRIBUTING TO THIS
  • 4. SCREENING PRINCIPLES Screening is done for: • Disorders with common prevalence • Have significant impact on perinatal mortality & morbidity Conditions to be fulfilled: • Accessibility, Availability , Affordability • Must understand Cost of burden of the disease vs cost of screening
  • 5. What Do Screening Tests Do? 1. Identify patients “at risk” for a disorder in an “unsuspected” population 2. “Filters” patients for further diagnostic testing 3. Results are given as “high risk” or “low risk” based on a “cut off” value
  • 6. PRENATAL SCREENING • I TRIMESTER • History, MAP, Ut A doppler / Biochem • II TRIMESTER(?) • UT A doppler • CERVICAL LENGTH – II trimester • I & II TRIMESTERS • ULTRASOUND • BIOCHEMISTRY • CELL FREE DNA • I & II TRIMESTERS ANEUPLOIDY ANOMALY PRE- ECLAMPSIA PRETERM BIRTH
  • 7. PRENATAL TESTING SCREENING TEST •Provides individual risk assessment •Advantages • Lowers the number of procedures done for diagnosis • Lowers the procedure related complications •Disadvantages • Non diagnostic • May miss target DIAGNOSTIC TEST •A test that WILL identify a disease or defect •Advantages • Definitive •Disadvantages • Risk associated with diagnostic procedure/s
  • 8. Magnitude of Problem Congenital & Genetic Disorders in India Disorder Frequency at birth in stillbirths in NN Deaths Congenital 2-5% (1:50 , 6 lacs/yr) 13.6 % 7 – 10 % Malformations Chromosomal 0.5% ( DS – 1:916 , 22,000 / yr ) Single Gene 0.6% ( B- thal – 1:2700 , 9000/ yr ; SCD - 5,200 /yr ; DMD + SMA - 4,500 / yr ) ( IC Verma , Preventive Genetics ,2006 )
  • 9. Chromosomal defects Source: Kagan KO et al. Screening for Chromosomal Abnormalities by First Trimester Combined Screening and Noninvasive Prenatal Testing. Ultraschall in Med 2015; 36:40-46)
  • 10. FOGSI OLD CHECK LIST OF 2009,MODIFIED IN 2017 AT FOGSI T.O.G.
  • 11. SCREENING FOR ANEUPLOIDY • Trisomy 21 - Down syndrome - 1 in 800 • Trisomy 18 – Edwards synd. - 1 in 10,000 • Trisomy 13 – Patau’s syndrome > 1 in 10,000 Apriori Risk MATERNAL AGE, Previous screening) Identify markers (USG, Biochem) Modify Risk Identify Patients for invasive testing
  • 12. 12 TEST FIRST TRIMESTER SECOND TRIMESTER CRL 45-84 BPD 30mm -51mm 10 11 12 13 14 15 16 17 18 19 20 Sequential Screen NT, PAPP-A, hCG +PLGF AFP, hCG, uE3, Inhibin A CONTINGENT SCREEN NB/ DV/TR Serum Integrated Screen hCG , PAPP-A AFP, hCG, uE3, Inhibin A Quad Screen E-FTS PAPP-A, hCG +AFP +PLGF AFP, hCG, uE3, Inhibin A 1 4 w G r a y Z o n e THE TIMELINES FOR SCREENING NIPS – after 10 weeks – ideal before 17 weeks to help decision making < 20 weeks
  • 13. First trimester screening FOR CHROMOSOMAL ANOMALIES FETAL CROWN FETAL RUMP NT/NB DV TR
  • 14. First Trimester Screening – The yield Test Name Time of Test(in Weeks) Markers DR(%) FPRs ( % ) Early Biochemistry 9-10^+6 MA+hCGB, PAPP-A ~60-65 5 % COMBINED FIRST TRIMESTER SCREENING 11-13^+6 MA+hCGB, PAPP-A+NT ~90-91 3 % 11-13^+6 MA+hCGB, PAPPA+NT +NB+tri cuspid flow+facial angle+Ductus Venoses ~95% 3 % Penta Screening 10- 13^+6 MA+ hCGB, PAPPA, PIGF, DIA+NT+NB 98 % 1.2 % BE HAPPY TEST
  • 15. JOGI – Feb 2019
  • 16. Objective • To derive a risk calculation algorithm suitable for use in India when screening for Down’s • Syndrome using four first-trimester maternal serum markers either alone or with ultrasound nuchal translucency (NT).
  • 17. Enhanced Combined test 1: 250 cutoff Enhanced Combined EFTS COMBINED TEST DETECTION RATE 90% 85% FALSE +ve rate 1.4% 1.8%
  • 18. Screening for Trisomy 21 at 11- 14 weeks 2-stage (contingency) screening- UK system COMNINED TEST (NT+BIOCHEM) FOR ALL Fetal NT and free BhCG and PAPP-A at 12 wks High risk >1:250 low risk <1:1000 CVS Reassure Borderline risk 1 in 251-1:1000 Further screening Nasal bone DV, TR NIPS
  • 19. 99
  • 21. Second Trimester Screening Screening Strategy Time of Test(in Weeks) Markers Used DR(%) FPRs ( %) Triple Test 15-21^+6 MA+AFP,hCGB, uE3 ~65-70 5-7% Quadruple Test 15-21^+6 MA+AFP,hCGB, uE3 ,Inhibin-A ~70-75 5-7% Integrated Test 15-21^+6 1st Trimester – PAPP-A 11-13+6/7weeks (11 Wks is Ideal) 2nd Trimester –Quad AFP, uE3, FBhCG, Inhibin-A (15-17 Wks is ideal) 93% 3 %
  • 22. Contingent II trimester “Genetic sonogram” To modify risks after FTS combined, Quadruple Or Integrated screening Needs high USG expertise Software for calculation ARSA Absent NB
  • 23. When there are major structural defects NO screening is offered – Direct testing is preferred
  • 24. SCREENING FOR FETAL ANOMALIES- I TRIMESTER 70% detection rate if a systematic scan is done
  • 25. Pre-Eclampsia • Adaptive disease when there is relative placental imbalance (Utero Placental mismatch) – Late onset may be beneficial to the baby – improved quality of survival in late mild PE • Early onset may have implications for mother / baby
  • 26. SCREENING FOR PE • Maternal history • Maternal blood pressure • Uterine artery doppler • Biochemical markers • Combination .. PAPP-A / PLGF
  • 27. First trimester screening for Preeclampsia Maternal serum PIGF, Mean arterial Blood pressure - Implantation - Maternal artery remodelling Detection rate – 90% 0 10 20 30 Falsepositive(%) Doppler 12% 30% PP13 9% Doppler & PP13
  • 28. History + MAP + UT A doppler + PLGF & PAPP-A • 93% detection rate (5% FPR) for early preeclampsia (<34 weeks) Poon LC et al Hypertension 2009 A combination of markers at 11- 13 weeks is ideal
  • 29. • Low-dose aspirin initiated in early pregnancy is an efficient method of reducing the incidence of preeclampsia and IUGR. (Obstet Gynecol 2010;116:402–14) Is there intervention??
  • 30. Is there intervention if screened in first trimester? • Low-dose ASA may prevent as many as 50% of cases of PE & IUGR when treatment is initiated before 16 weeks of gestation Bujold E, et al Obstet Gynecol 2010;116(2 Pt 1):402–14. Bujold E et al J Obstet Gynaecol Can 2009;31:818–26.
  • 31. DIAGNOSTIC TESTS AFTER SCREENING WHAT TO ORDER AND WHAT TESTS TELLS WHAT
  • 32. DIAGNOSTIC CONFIRMATORY TESTING AFTER SCREEN POSITIVE RESULT • What tests: –Karyotyping • Aneuplodies , structural rearrangements –Microdeletions • 22q most common –Microarray • Increased NT – Normal Karyotype • Deletions & duplications
  • 33. 1. Karyotyping 2. Fluorescence In Situ Hybridization (FISH) 3. Polymerase Chain Reaction (PCR) 4. Array‐based comparative genomic hybridization (array CGH) i.e. chromosomal microarray analysis (CMA) ,next-generation sequencing (NGS) , whole-exome sequencing Shaffer LG, Bui T‐H. 2007. Molecular cytogenetic and rapid aneuploidy detection methods in prenatal diagnosis. Am J Med Genet Part C Semin Med Genet 145C:87–98. Testing with foetal cells
  • 34. Karyotype can detect • Some specific abnormalities e.g. - Trisomies (21,18,13), Klinefelter's syndrome (XXY and other variations), Triple X syndrome (XXX) - Monosomy : Turner syndrome (X0) • Some Chromosomal deletions - Cri-du-Chat syndrome (missingCh5) - Williams syndrome (missing Ch7) • Translocations : Robertsonian translocations Limitation : Cannot detect specific gene mutations e.g. cystic fibrosis , Thalassemia. Resolution limited to around 5 Mb.
  • 35. Molecular cytogenetics :FISH (Florescence In Situ Hybridization) • Is a cytogenetic technique used to detect and localize the presence or absence of specific DNA sequences on chromosomes • Allows visualization of small region on chromosome too small to be identified by karyotyping(submicroscopic deletion) • Unlike Karyotype(21days) results available with in 24 to 72 hrs as done on interphase nuclei
  • 36. QF-PCR  has recently entered the field of prenatal diagnosis to overcome the need to culture fetal cells, allow rapid diagnosis of some selected chromosomal anomalies.  has the advantage of being much less expensive and allowing the simultaneous processing of much larger number of samples than FISH.  Can detect mosaicism of about 20–30% and is superior to both traditional karyotyping and interphase FISH for the identification of maternal cell contamination [ Donaghue et al., 2005]
  • 37. QF-PCR: Offerings QF-PCR BASIC QF-PCR EXTENDED Coverage • Trisomies :13,18,21 and Gonsomal Aneuploidies  Trisomies :13, 18,21, 15,16,22, Gonosomal Aneuploidies  20 common microdeletions and microduplications:  DiGeorge Syndrome,Langer- Giedons Syndrome,Smith- Magnenis Syndrome,Miller- Dieker Syndrome,Williams- Beuren Syndrome,Potoscki- Lupuski Syndrome
  • 38. Microarray Analysis Can identify chromosomal aneuploidy , large structure changes as well as submicroscopic abnormalities that are too small to be detected by traditional modalities A DNA microarray is a thin-sized chip that has been spotted at fixed locations with thousands of single- stranded DNA fragments corresponding to various genes of interest A single microarray may contain 10,000 or more spots, each containing pieces of DNA from a different gene
  • 39. Introduction of chromosomal microarray analysis into prenatal diagnosis • CMA is now the first-tier genetic diagnostic test for children and adults with multiple congenital anomalies, genetic syndromes, and intellectual and developmental disabilities, diagnostic yield - 15 to 20% • CMA is recommended as a primary test, by ACOG ,after USG finding of structural abnormality unless the abnormality is “strongly suggestive” of a particular aneuploidy • CMA suitable for analysis of stillbirth samples & early miscarriages , it does not require actively dividing cells Miller DT, Adam MP, Aradhya S, et al. Am J Hum Genet. 2010;86(5):749–64. Hillman SC, McMullan DJ, Hall G, et al. : Ultrasound Obstet Gynecol. 2013;41(6) ACOG Practice Bulletin,163:2016
  • 40. Next Generation Sequencing(NGS) • Sequence each of the 3 billion bases in the human genome multiple times providing an insight into unexpected DNA variation missed by other methods. • Can sequence entire genomes or specific areas of interest, including all 22 000 coding genes (a whole exome) or small numbers of individual genes • By providing a base-by-base view of the genome, NGS can identify single nucleotide variants (SNV), small structural changes, and balanced translocations • increasing information while decreasing costs with a genome-wide view of variation. Arch Dis Child Educ Pract Ed. 2013 Dec; 98(6): 236–238
  • 42. Whole-exome sequencing(WES) • Congenital abnormalities identified USG , karyotype and CMA reveal a diagnosis in up to 20–30%, for the remainder, single-gene tests or gene panels, may be useful • CMA and NGS based methods, such as targeted gene- panel sequencing and, recently, whole-exome sequencing (WES), has enabled to diagnose more fetal genetic conditions • In WES, majority of coding exons, which represent only 2% of the genome but contain 85% of disease-causing mutations, are sequenced Lee H, Deignan JL, Dorrani N, et al. : . JAMA. 2014;312(18). Gilissen C, Hehir-Kwa JY, Thung DT, et al. : Nature. 2014;511(7509) Beaulieu CL, Majewski J, Schwartzentruber J, et al. : . Am J Hum Genet. 2014;94(6)
  • 43. Cont-- • The American College of Medical Genetics and Genomics recommends considering WES when specific genetic tests available for a phenotype, including targeted sequencing , have failed to determine a diagnosis in a fetus with multiple congenital anomalies suggestive of a genetic disorder • Routine use of whole-genome or whole-exome sequencing is not recommended outside of the context of clinical trials ACMG Board of Directors. Genet Med 2012;14:759–61 , ACOG Practice bulletin ,Number 682, December 2016
  • 44. Take home message SCREEING SHOULD BE OFFERED TO ALL POPULATION IRRECPECTIVE OF RISK While • Testing should be focused on the individual patient's risks, reproductive goals, and preferences Patients should understand the benefits and limitations , including the conditions that will not be detected by tests PRE AND POST TEST COUNCELLING IS VERY IMPORTANT
  • 45. Various Integrated screening in strategies (1st and 2nd trim) Main strategies: • Fully Integrated • Step-wise sequential • Contingent screening 1st trimester: NT, PAPP-A No risk estimate 2nd trimester: Fb-hCG, AFP, uE3, (± Inhibin) Final risk estimate: All markers 1st trimester: NT, PAPP-A, Fb-hCG Risk estimate Final risk estimate: All markers CVS NIPT High risk Low risk 2nd trimester: Fb-hCG, AFP, uE3, (± Inhibin) 1st trimester: NT, PAPP-A, Fb-hCG Risk estimate 2nd trimester: Fb-hCG, AFP, uE3, (± Inhibin) Final risk estimate: All markers CVS NIPT HR Borderline risk No further screening LR
  • 46. Thank you Screen with the right test at the right time