Lecture 10

Question 1

in what situation do we use a cytogenic approaches instead of molecular approaches?

Answer 1

if we have very big alterations, insertions or deletions of different mega bases at the chromosomal level

Question 2

what do we used of there are only small insertions or deletions of a few megabases or if there is the lacking of one entire exon?

Answer 2

classical PCR

Question 3

what can the intrinsic bias of classical PCR cause?

Answer 3

allele dropout → during the amplification exploiting the classical PCR, there is the design two different primers (forward and reverse), and after the annealing there is
the elongation and the copy of the target of interest: if there is an alteration, for example a heterozygous deletion, there will be the annealing of only one primer and not the complete amplification, resulting in the amplification of only one allele, while the other one will be not amplified → we are not able to detect that lack of amplification

Question 4

what are the three approaches used for the identification of insertions or deletions at the gene level?

Answer 4

1. multiplex PCR of short fluorescent fragments (MPSF)
2. multiplex amplification and probe hybridization (MAPH)
3. multiplex ligation-dependent probe amplification (MLPA)

Question 5

what has MPSF been developed to detect?

Answer 5

large insertions and deletions on two genes (MLH1 and MLH2) which are mismatch reaping genes associated with hereditary non-polyposis colorectal cancer

Question 6

describe MPSF:

Answer 6

a quantitative method based on the multiplex amplification of all exons composing the specific gene exploiting probes labelled with fluorescence → we amplify different regions of the gene in the same run or analysis exploiting the use of fluorescent fragments

Question 7

how many primers are used for MPSF?

Answer 7

two, in order to reduce the difference occurring during the amplification and to have the same amplification for all regions the gene in the same run

Question 8

what is mandatory in MPSF analysis?

Answer 8

to have a wild type as a control analyzed in the same run and at the same time as out samples

Question 9

what does it mean if the peak of the sample is higher than the wild type?

Answer 9

there’s a duplication

Question 10

what does it mean if the peak of the sample is lower than the peak of the wild type?

Answer 10

there is a deletion

Question 11

what type of deletion occurs if the reduction of the peak area is 0.5?

Answer 11

a heterozygous deletion

Question 12

what does it mean if the increase in peak area is 1.5?

Answer 12

there is a heterozygous duplication

Question 13

STUDY EXAMPLE FOR MPSF

Answer 13

pg 2-3 sbobine

Question 14

in order to exploit the MPSF approach, with is required?

Answer 14

a large amount of starting DNA → also important to extract all that DNA in the exact same way to avid contamination due to different approaches of extraction

Question 15

what type of approach is MPSF and what is the main idea?

Answer 15

quantitative → comparison of the sample with the control based on multiplex amplification of different regions of interest

Question 16

what was QMPSF created for?

Answer 16

modified version of MPSF for the analysis of particular kinds of genes:
- genes characterized by the presence of GC regions (difficult to amplify)
- for pseudogenes (regions of he genome with high homology with the genes

Question 17

how id QMPSF modified in order to find certain genes?

Answer 17

modified primer → the primer for the amplification presents an extension of 6 nucleotides in the 5’, a TAG, which is not complementary to the target region, but is only useful to have similar sizes of the amplicon, to have the same amplification at the same time of all the exons.
It is similar to the previous approach because the primers are labelled with fluorescence and there is
also the amplification of the wild type together with the sample. After the analysis on the sequencer, we obtain different peaks with different colours in the wild type and in the mutated sample, and it is possible to compare the area of each peak

Question 18

REVIEW QMPFS

Answer 18

pg 4-5

Question 19

with QMPFS, can we confirm the result, because with a a deletion we are sure that the primers were designed very far away, so are you able to create a fragment?

Answer 19

yes : you know where the deletion is so you can design the primers in the adjacent region

Question 20

in QMPFS, is there a specific reason why the exons are not in order in the graphical representation?

Answer 20

it depends on the feature of the region and on the amplification condition of different exons - in this case you don’t have one single multiplex, but it is necessary to have four different multiplexes for the BRCA1 because it is a difficult gene to amplify using PCR

Question 21

what are the main features of MAPH?

Answer 21

it allows us to analyzed up to 40 loci at the same time, or to analyze a big gene entirely in the same analysis

Question 22

how does MAPH work?

Answer 22

the DNA is hybridized with the specific probes in the target region, however it is not amplified, there willl only be an indirect amplification of the probes hybridized to the target region

Question 23

what do the probes in MAPH correspond to?

Answer 23

a specific region - it is necessary to consider the height of the peaks → if there is a reduction we have a deletion, and if there is a higher peak then we have a duplication

Question 24

what is one of the limitations of MAPH?

Answer 24

there is a possibility for a heterogenous condition for the hybridization of DNA on the nylon, on the solid support, and therefor the loss of the hybridized probes during washes → results in the detection of non-existent deletions

Question 25

what is MAPH characterized by?

Answer 25

indirect amplification

Question 26

what is the main advantage of MAPH?

Answer 26

we can analyze different loci and very big genes

Question 27

how is MLPA different than MAPH?

Answer 27

we still have the amplification of the probes and not the DNA, but we have the hybridization and amplification in solution

Question 28

describe the primers in MLPA:

Answer 28

a couple of primers: the primer is complementary to the target region, and in the flanking region we gave tw universal primers that are necessary for the amplification; we also have the “stuffer region”: characterized by a variable length of several base pairs and is composed of nucleotides

Question 29

what are the amplicons generated by MLPA characterized by?

Answer 29

characterized by different sizes depending on the stuffer region that is incorporated / amplified

Question 30

what occurs in MLPA if there is a homozygous deletion?

Answer 30

no amplification

Question 31

what occurs in MLPA if we have a heterozygous deletion?

Answer 31

amplification of one allele and we will have different peaks for different regions

Question 32

what do we use as a control of MLPA?

Answer 32

deleted sample as well as a WT → NOT an absolute quantification because we need a control for comparison

Question 33

what does MLPA allow us to do?

Answer 33

analyze several loci simultaneously at the chromosomic or genic level

Question 34

what must we keep in mind when creating / analyzing controls?

Answer 34

the female has 2X chromosomes so there will be a higher peak

Question 35

how do we analyze MLPA at the gene level?

Answer 35

we analyze the heights of each peak

Question 36

what are MLPA and MLPH based on?

Answer 36

indirect amplification (probes)

Question 37

what is an important difference between MLPA and MLPH?

Answer 37

the amount of DNA needed for analysis:
- for MLPH we need 1µg (very large and not always possible to obtain)
- for MLPA we need 100-200 ng

we also have commercial kits for MLPA that have been validated and commercialized

Question 38

which is more commonly used, MLPA or MLPH?

Answer 38

MLPA: it is widely used and overcomes the limitations of MLPH → it allows us to identify low-level somatic DNA mutations and minority alleles

Question 39

what is PNA?

Answer 39

peptide nucleic acids → one of the first approaches developed for minority allele identification

Question 40

what is PNA characterized by?

Answer 40

a good ability to hybridize DNA and RNA - also chemical structure that has a very high stability and it mimics DNA (entire backbone is sugar phosphate is replaced with a neutral backbone consisting of repeated units of N-glycine)

Question 41

how does the PNA interact with DNA?

Answer 41

it is able to hybridize a DNA strand if there is the same complementary criteria between bases

Question 42

describe PNA stability:

Answer 42

stability between PNA and DNA is higher than DNA-DNA

Question 43

what happens if we have the PNA structure hybridized on the DNA strand?

Answer 43

amplification is NOT possible

Question 44

what can we design a PNA complementary to?

Answer 44

a WT sequence → we have to set the PNA concentration required to reduce the number of WT molecules that are amplified

Question 45

when dealing with PNA and WT sequences, what is the goal?

Answer 45

we must find the best PNA concentration that allows for the reduction of the amplification of the WT molecule k

Question 45

what was developed through PNA?

Answer 45

the first non-invasive prenatal diagnostic tool

Question 46

when dealing with an autosomal mutation in a baby, how can we design the PNA?

Answer 46

for the specific region in which the mutation is located → we can focus our analysis not specifically on that mutation, but on a polymorphism close to the mutation that is different in the mother and the father → we can have an indirect analysis focusing on the polymorphism and not on the direct mutation

Question 47

what is the great advantage of PNA?

Answer 47

after the amplification the amplicon we obtain can be analyzed using different approaches

Question 48

what are the two main limitations of PNA?

Answer 48

1. we have to know exactly where the mutation is
2. every time we have to establish the best concentrations needed to be sure that we can detect the allele

Question 49

besides prenatal testing, what can PNA be used for?

Answer 49

detection of KRAS mutation

Question 50

what has PNA been superseded by?

Answer 50

droplet digital PCR