Bocian Chromosome Structure and Variation

Question 1

Describe chromosome morphology

Answer 1

Two arms connected at the centromere

Question 2

Arms of a chromosome

Answer 2

Short arm = p

Long arm = q

Question 3

Three general shapes of a chromosome

Answer 3

a) Metacentric (centromere is in the middle)
b) Submetacentric (centromere is off-center)
c) Acrocentric (centromere is near the end)

Question 4

Acrocentric chromsomes have?

Answer 4

Satellites at the top end of the short arm

Code for rRNA and are called Nucleolar organizing regions

Question 5

Ends of chromsomes are claled?

Answer 5

The ends of the chromosomes are called telomeres; the small portions just next to the
telomeres are called the sub-telomeric regions.

Question 6

Chromosome during the cell cycle (early and after replication)

Answer 6

Each chromosome consists of 1 chromatid in early cell cycle and two sister chromatids after
replication (but before cell division)

Question 7

Number of chromosomes in normal human somatic cell

Answer 7

46 chromosomes (23 pairs)

Question 8

What are homologus chromosomes?

Answer 8

Each pair consists of one maternally-derived and one paternally-derived chromosome
(homologs or homologous chromosomes)

Question 9

What are autosomes?

Answer 9

22 pairs of chromosomes, non-sex chromsomes

Question 10

Sex chromosomes number?

Answer 10

1 pair of sex chromosomes (XX or XY)

Question 11

What is a Karyotype?

Answer 11

conventional arrangement of metaphase chromosomes for analysis

Question 12

Cells must be what to do a Karyotype?

Answer 12

Cells must be living and dividing in order to get metaphase chromosomes to construct and analyze a karyotype

a) Samples are grown in tissue culture to obtain dividing cells (therefore, you cannot freeze samples, or place them in preservatives such as formalin, or get them contaminated with bacteria, or let them dry out, etc.)

Question 13

Common type of sample for individual chromosome Karyotype

Answer 13

To study an individual’s chromosomes: blood lymphocytes (a type of white cell) are by
far the most commonly used

Question 14

Common type of sample for karyotype of fetus

Answer 14

To study the chromosome of a fetus: amniotic fluid (contains fetal epidermal cells) is by
far the most commonly used; also, chorionic villi (placental cells)

Question 15

Common type of sample for the karyotype of tumors

Answer 15

Bone marrow, tumor tissue

Question 16

What must be added to do a karyotype? What is used for lymphocytes?

Answer 16

Must add a mitogen (i.e., an agent that causes mitosis) for blood lymphocyte cultures (phytohemagglutinin—stimulates lymphocytes to divide)

Question 17

What is added to accumulate cells in metaphase for a karyotype?

Answer 17

Colcemide – a compound related to colchicine - destroys the mitotic spindle

Question 18

What is Banding?

Answer 18

Each chromosome has a unique sequence of bar code-like stripes, allowing
identification of individual homologs and the analysis of abnormalities of their structure by
disruption of the normal banding pattern

Question 19

Describe the staining of G-(Giemsa) Banding. What is dark? Light?

Answer 19

AT-rich regions stain (G-dark bands); GC-rich regions do not stain (G-light bands)

Question 20

Describe high resolution analysis of chromosomes (high res karyotype)

Answer 20

Chromosomes are prepared in prometaphase (or even late prophase) instead of metaphase to make them longer and increase the number of sub-bands that can be seen

Question 21

Compare routine and high res karyotype

Answer 21

Routine can see 450-500 bands

High res caan see 550-800 bands

Question 22

Each chromosome is divided into what notationally?

Answer 22

Divided into standard regions

Question 23

Describe the numbering of chromosome regions

Answer 23

The regions are numbered, in order, from the centromere toward the ends
a) e.g., the long arm (q) of chromosome 1 consists of four regions numbered consecutively
from the centromere outward: 1q1, 1q2, 1q3, 1q4

The regions are further subdivided, e.g. 1q11, 1q12, 1q13, etc.
a) Then further subdivision: 1q11.1, 1q11.2, etc.

Question 24

Give examples of chromosome cytogenetic shorthand notation

Answer 24

a) 46,XY
(1) 46 chromosomes total, with one X and one Y (a normal male karyotype)

b) 46,XX
(1) 46 chromosomes total, with two Xs (a normal female karyotype)

c) 47,XY,+21
(1) 47 chromosomes total, with an X and a Y and an extra (+) chromosome #21

d) 45,XX,-22
(1) 45 chromosomes total, with two X’s and a missing (-) chromosome #22

Question 25

Describe how to write out chromsomes with duplication, deletion, and translocation in shorthand notation

Answer 25

e) 46,XY,dup(7)(q11q31)
(1) 46 chromosomes total with an X and a Y; there is a duplication of the material on the
long arm of chromosome 7 from region q11 to region q31

f) 46,XY,del (22)(q11.2)
(1) 46 chromosomes total with an X and a Y; one of the chromosomes #22 is missing a
portion of the long arm located at region q11.2 (del = deletion)

g) 46, XX, t (7;9) (p21.2;q34.1)
(1) A female with a balanced translocation, i.e., an even exchange [more about this
below] of portions of chromosome 7 starting at 7p21.2 and chromosome 9 starting at
9q34.1

Question 26

Karyotype results should state the?

Answer 26

Band level (the resolution)

Question 27

Molecular cytogenetics are used to detect?

Answer 27

Deletions of duplications smaller than 4 Mb

A DNA probe is used to detect the presence or absence of a specific chromosomal
segment

Question 28

What can be detected by molecular cytogenetics?

Answer 28

A DNA probe is used to detect the presence or absence of a specific chromosomal
segment

Chromosomal abnormalities can be detected in both dividing and non-dividing cells

Question 29

What is FISH?

Answer 29

FISH (Fluorescence In Situ Hybridization)

Identification of specific chromosomes and parts of chromosomes by in situ hybridization with labeled DNA probes

Question 30

FISH is useful for (5 things)?

Answer 30

(1) Detecting submicroscopic deletions and duplications
(2) Detecting subtle chromosome rearrangements
(3) Identifying marker chromosomes (see definition below)
(4) Identifying the content of multiple rearranged chromosomes
(5) Detecting aneuploidy (extra or missing chromosomes) in interphase cells in
cancers

Question 31

3 types of FISH used in clinical studies

Answer 31

Centromeric probes
Whole Chromosome Paint probes
Unique sequence probes

Question 32

Describe centromeric FISH probes

Answer 32

Centromeric probes (Satellite repeat-sequence probes)

(a) Target only the centromeres of specific chromosomes

(b) Useful in determining the number of chromosomes in cases of possible
aneuploidy syndromes (disorders due to extra or missing chromosomes) or in cancer cells

(c) Can use with interphase cells if metaphase cells are not available

Question 33

Describe whole chromosome paint FISH probes

Answer 33

Cover an entire chromosome

Used as a screening tool in the characterization of an abnormal chromosome.

Question 34

Describe unique sequence FISH probes

Answer 34

Target a specific locus (or gene) on a chromosome

(b) Use for diagnosis of chromosome microdeletion or microduplication
syndromes

(c) Certain acquired translocations that are unique to specific cancers can be
detected in interphase cancer cells with dual-color unique sequence probes.

Question 35

Describe FISH nomenclature

Answer 35

Capital letters and numbers are used for the locus, and “+” or “−” given immediately afterward indicates whether the locus has been identified as being present or absent,respectively.

Question 36

Describe subtelomere analysis

Answer 36

FISH analysis of individuals with idiopathic (i.e., unexplained) intellectual disabilities, with
or without congenital malformations, shows that a significant proportion (5-10%) of these
patients have unbalanced abnormalities involving the subtelomeres. Many or most (~50%)
of these abnormal subtelomere cases are familial (i.e., inherited from a carrier parent),
which has important implications for genetic counseling and recurrence risk estimates.

Question 37

Describe Chromosomal microarray analysis

Answer 37

A very high-resolution molecular cytogenetic technique that is used to detect
submicroscopic chromosomal duplications and deletions (copy number variants, CNVs).

A series of DNA or RNA probes is placed on a glass slide or silicon wafer (chip) and
hybridized with DNA or RNA from the patient

Question 38

Three types of Chromosomal microarray analysis

Answer 38

Genomic Array
Expression Array
Molecular probe inversion array

Question 39

Describe genomic array chromosomal microarray analysis

Answer 39

(i) DNA-based

(ii) Looks for changes (loss or gain) in a patient’s DNA

Question 40

Describe expression array chromosomal microarray analysis

Answer 40

RNA-based

(i) Looks for expression of a series of genes
(ii) Often used in cancer profiling

Question 41

What is array-based comparative genomic hybridization (array CGH)

Answer 41

Compares a sample of patient’s DNA to normal control DNA…..by observing their ability to compete with each other for hybridization to an array of thousands of reference DNA probes immobilized on a slide or chip

Question 42

Array CGH tells us?

Answer 42

Copy number variations (CNV) are determined by the differences in hybridization pattern intensities between patient DNA and control DNA. The copy number of each clone (i.e., how many copies of that clone determined based on the ratio of the hybridization signal between the patient’s DNA and normal control DNA for each chromosome

Question 43

What is a copy number variation?

Answer 43

In Array CGH

A copy number variation (CNV) is a segment of extra or missing DNA
detected by microarray analysis

Question 44

Normal CNV in a CGH tells us?

Answer 44

Normal: The amount of patient DNA equals the amount of control DNA (1:1 ratio of patient to control DNA)

Question 45

CNV in a CGH with duplication?

Answer 45

Duplications of chromosomes in patient DNA result in favorable hybridization of the patient sample to the spots on the array (ratio 1.5 patient DNA : 1 control DNA)

Question 46

CNV in a CGH with deletion?

Answer 46

Deletions of chromosomes in patient DNA result in favorable hybridization of the normal DNA to the spots on the array (ratio 0.5 patient DNA : 1 control DNA)

Question 47

Array resolution of a CGH depends on?

Answer 47

Array resolution depends on probe size and spacing along the genome and by the
specific statistical algorithms used to set the criteria for gains and losses.

Question 48

Describe the three types of CGH

Answer 48

Comparative using Bacterial artificial chromosome arrays or oligonucleotide arrays

Single nucleotide polymorphism arrays

Question 49

Describe targeted probes for CGH

Answer 49

Targeted probes: Uses probes mainly from specifically defined regions of known
microdeletion or duplication syndromes and all centromeric and telomeric regions

Question 50

Describe constitutional probes for CGH

Answer 50

Uses probes from the entire genome
(including the centromeric and telomeric regions), relatively evenly-spaced across
the genome, e.g. fragments spaced at 1 Mb intervals or 300 kb intervals throughout
the genome, or they may use overlapping (contiguous) clones

Question 51

Compare the accuracy of an oligo array and a BAC array for CGH

Answer 51

copy number changes that were missed on a BAC array – therefore, if a patient had a normal BAC array in the past, an oligo array (or a SNP array) may pick up an abnormality that was missed on the BAC array.

Question 52

What is a SNP?

Answer 52

A single nucleotide polymorphism (SNP), a variation at a single site in DNA, is the
most frequent type of variation in the genome.

Question 53

A SNP is what genetically?

Answer 53

A SNP has a single base pair substitution (A, T, C, or G) of one nucleotide for another

But it’s not considered to be a mutation
(“Polymorphism” = normal population variant

Question 54

What is the criteria to be a SNP?

Answer 54

To be considered a SNP, the substitution must be found in at least 1% of the general population

Question 55

Where can SNPs occur?

Answer 55

SNPs can occur within the coding sequence of a gene, the non-coding regions of genes,
or the inter-genic regions (between genes)

Question 56

What do SNP arrays detect?

Answer 56

Copy number changes, and also……….

Certain types of copy-neutral changes (no change in copy-number) that are not
detected by CGH arrays:
(a) Can detect long contiguous stretches of homozygosity (hmz) (LCSH) that are associated with uniparental disomy or with consanguinity or incest, each of which increases the risk for autosomal recessive disorders

Question 57

Describe what SNP arrays are really good at detecting?

Answer 57

This advantage of SNP arrays has a huge potential in cancer diagnostics, since loss of heterozygosity (LOH) is a prominent
characteristic of most human cancers. LOH is a form of allelic imbalance that can result either from the complete loss of an allele (by
deletion) or from UPD (uniparental disomy, in which an individual
has two copies of certain stretches of genes from one parent and no
copies from the other parent)

Question 58

SNP arrays can detect what type of genetic disorder?

Answer 58

Triploidy (extra copy of every chromosome)

Question 59

Difference between SNP and CGH?

Answer 59

SNP arrays differ from CGH arrays in that only the patient’s genome is hybridized to the slide (do not need a control patient’s DNA)

Question 60

Copy number assesssment of SNP and CGH?

Answer 60

SNP arrays allow a more comprehensive assessment of copy number than CGH arrays

Question 61

What is B allele frequency?

Answer 61

Metric provided by SNP array

B allele frequency (BAF) is the proportion of the total allele signal (A+B) explained by a single allele (A)

BAF can detect copy numbers from 0 to 4

Question 62

How is microarray diagnoses written? Normal male? Normal Female?

Answer 62

Female arr(1–22)x2,(X)x2
Male arr(1–22)x2,(XY)x1

Question 63

Examples of microarray deletions or duplications?

Answer 63

(1) For example, a 698 kb interstitial duplication in chromosome 1q43:
(a) arr 1q43(241,822,181-242,519,964)x3 [hg19]
(2) Another example: an interstitial deletion of the short arm of chromosome 20:
(a) arr 20p12.2(10,454,698–10,818,327)x1 [hg19]. This specifies a 323,630 bp
(324 kb) deletion within chromosome 20p12.2.

The (numbers) are molecular coordinates related to the location of base pair on
the gene map and can be used to look up genes within that segment and to
compare features of other patients with overlapping copy number variations

[hg19] refers to the version gene map that was used to interpret this analysis

Question 64

CNV can be?

Answer 64

Microdelections or microduplications (not SNPs)

Question 65

Describe the types of CNV?

Answer 65

Everyone has CNV

Pathogenic
Benign
Variants of unknown clinical significance

Question 66

Are CNV typically helpful?

Answer 66

Often the CNV are not easy to interpret

Question 67

Microarray advantage over karyotype?

Answer 67

Provides analysis at much higher resolution than karyotyping. Detects an additional 5-20% of patients with unexplained intellectual disabilities and/or congenital anomalies (compared with those who have had normal karytoype
analysis and subtelomere FISH analysis)

Question 68

Microarray advantage for supply material?

Answer 68

Uses DNA - does not need cultured, dividing cells

Question 69

Array CGH data compared to FISH?

Answer 69

Array CGH provides the equivalent of multiple, concurrent FISH analyses over hundreds or thousands of loci

(a) Single-probe FISH requires clinical suspicion of a specific disorder so that the correct probe(s) can be used

Question 70

Microarray correlation with phenotype?

Answer 70

Allows correlation of phenotype with genes (deleted or duplicated) in the affected region

(a) Inclusion of the genomic coordinates for each of these abnormalities allows the laboratory or physician to go to the genomic databases to determine the precise gene content of the deletion or duplication.
(b) Allows more precise characterization of imbalances, providing a better analysis of the phenotype

Question 71

Balances on Microarray versus karyotype?

Answer 71

Microarray can identify imbalances at the breakpoints of translocations that on karyotype analysis appear to be balanced and may even identify gene disruptions at the places where the chromosome(s) have broken

Question 72

SNP arrays can detect what that CGH cannot?

Answer 72

SNP arrays can identify UPD (isodisomy), consanguinity or incest, polyploidy (CGH arrays cannot identify these)

Question 73

Microarray analysis can tell us what about cancer?

Answer 73

the unexpected finding of tumor susceptibility

Question 74

What type of information does microarray not tell us?

Answer 74

do not provide any further positional information

regarding the imbalance.

Question 75

Array CGH cannot differntiate what?

Answer 75

Array CGH cannot differentiate free trisomies from unbalanced Robertsonian translocations

Question 76

CGH can tell us copy number variation relative to what?

Answer 76

The ploidy level of the reference DNA

Question 77

Microarray does not detect what type of chromosome anomaly?

Answer 77

Does not detect balanced chromosome anomalies (i.e., abnormalities in which
pieces of chromosomes have been moved around but are neither lost nor gained)

Question 78

Regions that are not represented on a microarray are?

Answer 78

Not assayed

Question 79

Describe limitation of microassay interpretation

Answer 79

Some of the changes it identifies are benign DNA variations (polymorphisms);
others are VUS that cannot be interpreted yet

Question 80

Microarrays and small base-pair duplications/deletions?

Answer 80

Array CGH cannot detect very small base-pair duplications or deletions (but
these can be detected by SNP array) or point mutations

Question 81

Triploidy and microarray?

Answer 81

Triploidy will not be detected by some forms of microarray (Yes in SNP and No in CGH)

Question 82

Aneuploidy and microarray?

Answer 82

Some aneuploidies can be missed, such as XYY if the wrong gender control is used.

Question 83

Marker chromsomes and microarray?

Answer 83

Marker chromosomes may also be missed, depending on the size, the composition of the marker, and whether there is good coverage in the array of the specific chromosomal region present on the marker.

Question 84

Microarrays and mosaicism?

Answer 84

The accuracy of detecting low levels of mosaicism (≤5-10%) is still in question

Question 85

Test for whether whole extra or missing chromsome?

Answer 85

Use routine karyotype

Question 86

Test for suspected specific, well-described microdeletion or microduplication

Answer 86

Use single-probe FISH analysis if a specific, well-described microdeletion or microduplication syndrome is suspected (e.g., Williams syndrome or the 22q11.2 deletion)

Question 87

Test for looking for a balanced translocation?

Answer 87

Use karyotype analysis ± FISH in cases where you are looking for a balanced translocations (microarray will not detect them because DNA is neither gained nor lost)

Question 88

When to use CGH or SNP array?

Answer 88

Use array CGH or SNP microarray as the first test in patients with multiple congenital anomalies and/or with unexplained intellectual disabilities if you don’t recognize the diagnosis, or when standard studies (karyotype, FISH) have not provided a diagnosis in patients suspected of being chromosomally abnormal

Question 89

Microarrays have markedly increased ability to do? (5 things)

Answer 89

(1) Find new microdeletion and microduplication syndromes
(2) Further delineate known syndromes
(3) Identify genes responsible for genetic disorders (candidate genes within duplicated or deleted regions)
(4) Detect mosaicism
(a) may miss low-level mosaicism
(5) Detect uniparental disomy (UPD) and consanguinity (SNP arrays)

Question 90

When should parental studies be done?

Answer 90

For pathogenic deletions and duplications, parental studies (by FISH or metaphase
preparations, if possible) should be conducted to rule out the presence of a chromosomal rearrangement such as an insertion or inherited duplication. Although these are rare, for a family in which such a rearrangement is found, recurrence risk can be as high as 50%

Question 91

What is Cell-Free Fetal DNA screening?

Answer 91

Analyzes circulating cffDNA from maternal blood in women at increased risk for fetal aneuploidy

1. Source of cff DNA:
   a) Placental cells break down, and fetal DNA enters maternal circulation
   b) ~10% of circulating DNA in maternal plasma is fetal

Question 92

What does ploidy mean?

Answer 92

“Ploidy” – Having to do with entire sets of chromosomes

Question 93

What is haploid

Answer 93

Haploid – 23 chromosomes

Question 94

What is euploid?

Answer 94

Euploid – Any number of chromosomes that is an exact multiple of the haploid number

Question 95

What is aneuploid?

Answer 95

Aneuploid – Cells deviating from the multiples of the haploid number are called aneuploid
(i.e., not euploid), indicating a missing or extra chromosome (e.g., 47 or 45 chromosomes)

Question 96

What is diploid?

Answer 96

Diploid - 46 chromosomes (23 pairs present) (“di” = 2 sets)(2n)

Question 97

What is polyploid?

Answer 97

Polyploid – having more than the normal two haploid sets of chromosomes:

Question 98

What is triploid?

Answer 98

Triploid – 69 chromosomes (an extra chromosome in each pair) (“tri” = 3n)

Question 99

What does somy mean?

Answer 99

Having to do with a single chromosome

Question 100

What is nullisomy?

Answer 100

both copies of the chromosome are missing (a non-viable state)

Question 101

What is monosomy?

Answer 101

A missing chromosome (e.g., monosomy-22, which means 45 chromosomes total
with only one chromosome #22)

Question 102

What is trisomy?

Answer 102

an extra chromosome (e.g., trisomy-21, which means 47 chromosomes total with three chromosomes #21)

Question 103

What is meant by constitutional chromosomal abnormality?

Answer 103

A chromosome abnormality that is present from conception or early fetal development and
involves the entire body

Question 104

Describe what is meant by acquired chromosome abnormality

Answer 104

New or added. “New” in the sense that it was not inherited, and “added” in the sense that it was
not congenital (present at birth) but came along later; usually used with respect to tumor or
cancer cells.

Acquired chromosome abnormalities are important in analyzing cancer cells

Question 105

What is a numerical chromosome abnormality?

Answer 105

An abnormality in the number of chromosomes present

1. May be constitutional or acquired
2. This is where you use the “ploidy” or “somy” terms

Question 106

What is a structural chromosome abnormality?

Answer 106

Structural chromosome abnormalities – An abnormality in the structure of one or more of the
chromosomes

“Somy” also may be used here, but it is usually used along with the word, “partial,” e.g., partial
trisomy of chromosome 8, which means that only a part of chromosome is duplicated

Question 107

What is mosaicism?

Answer 107

One or more additional cell lines with different chromosome complements arise in embryonic or pre-embryonic life and become an integral part of the organism; the individual has more than one kind of cell, e.g., some normal cells and some cells with trisomy 8

Question 108

What is a chimera?

Answer 108

Individuals with 2 or more cell lines, due specifically to the fusion of originally separate zygotes

Question 109

What is polyploidy?

Answer 109

Abnormalities involving the entire chromosome complement (sets of
chromosomes)

Question 110

What is triploidy? What does it result from?

Answer 110

Triploidy: 3 sets of chromosomes (3n=69); may be 69,XXX, 69,XXY, or 69,XYY.

Triploidy can result from dispermy (the extra set comes from the father) or digyny
(the extra set comes from the mother).

Question 111

What is tetraploidy?

Answer 111

Tetraploidy: 4 sets of chromosomes (4n); may be 92,XXXX or 92,XXYY

Question 112

Numerical abnormality involving a single chromosome is often from?

Answer 112

Usually result from meiotic non-disjunction (failure of homologous chromosomes to
separate symmetrically at cell division) occurring in egg or sperm. Infrequently due to
mitotic non-disjunction in the zygote. After non-disjunction, one daughter cell has an
extra chromosome and the other daughter cell has a missing chromosome.

Question 113

Example of a monosomy?

Answer 113

45,X (Turner syndrome)

Question 114

Examples of Trisomy?

Answer 114

(i) Trisomy 21 (Down syndrome)
(ii) Trisomy 13 (Patau syndrome)
(iii) Trisomy 18 (Edwards syndrome)

Question 115

Examples of sex chromosome trisomy?

Answer 115

(i) 47,XXY (Klinefelter syndrome)
(ii) 47,XXX (Triple-X syndrome)
(iii) 47,XYY syndrome (has no other name)

Question 116

Age of mother and correlation to type of chromosome abnormality?

Answer 116

The incidences of autosomal trisomy and of sex chromosome trisomy (XXY and XXX but not XYY) in offspring increase with the age of the mother, but the incidences of monosomy, polyploidy, and structural changes do not.

Question 117

Describe chromosomal mosaicism

Answer 117

The coexistence, within one embryo, of two or more distinct cell lines that are genetically identical except for the chromosomal difference between them. The different cell lines are established by the time embryonic development is complete (the point at which the embryo becomes a fetus), are fixed in the individual, and are part of his/her chromosomal constitution. There may be more than one cell line within a single tissue (e.g., two different cell lines found in the blood) or different cell lines among different tissues (e.g., one type of cell in the blood and another type of cell in the skin).

Notation: 47,XY,+21[8]/46,XY[42] denotes an individual in whom a total of 50 cells were
examined; [8] cells had an extra chromosome #21, and [42] cells were normal.

Question 118

What is somatic mosaicism?

Answer 118

the body consists of more than one type of cell

Question 119

What is germ line mosaicism?

Answer 119

the mosaicism exists in the eggs or sperm (sometimes also called
gonadal mosaicism)

Question 120

What is placental mosaicism?

Answer 120

Placental mosaicism, or confined placental mosaicism – About 1-2% of placentas have a
different chromosome constitution from that of the embryo; usually the embryo is normal
and the placenta is trisomic, but one or both can be mixed.

Question 121

What is trisomy rescue?

Answer 121

A trisomic zygote or early embryo loses the extra chromosome and becomes normal with respect to the number of chromosomes in each pair

Question 122

Structural abnormalities due to chromosomal rearrangements occur when?

Answer 122

can occur either during meiosis (more

common) or mitosis (less common)

Question 123

What are normal chromosomal heteromorphisms?

Answer 123

Normal chromosome heteromorphisms (“polymorphisms”) - Normal variations that are not associated with phenotypic abnormality and that usually are also found in one of the normal parents of the individuals in whom they occur

Question 124

Describe deletion

Answer 124

A portion of a chromosome is missing

Notation: 46,XY,del(22)(q11.2). The q11.2 segment is missing from one of the
chromosomes 22.

Question 125

What is a partial monosomy? Cryptic translocation?

Answer 125

Results in partial monosomy for the deleted segment

1) May be a cryptic translocation (“hidden” - too small to be seen without FISH

Question 126

Once a deletion is diagnosed, what must be done?

Answer 126

Once a deletion (or any other type of structural change) is diagnosed, you must rule
out a rearrangement in one of the patient’s parents

Question 127

What is microdeletion?

Answer 127

Microdeletion – The deletion is so small it cannot be seen by
conventional microscopic methods; a cryptic deletion. FISH or other
molecular techniques must be used to diagnose it. A microdeletion often
includes several gene loci.

Question 128

List three examples of autosomal microdeletions

Answer 128

(a) Williams syndrome (del 7q11.2)

(b) Prader-Willi syndrome — due either to del 15q11-q13pat (i.e., deletion ofna small portion of the chromosome #15 that was inherited from the
father) or to maternal UPD 15 (UPD = uniparental disomy and will be explained in your lecture on nontraditional inheritance)

(c) Angelman syndrome — due either to del 15q11-q13mat (i.e., deletion of a small portion of the chromosome #15 that was inherited from the mother) or to paternal UPD 15 (also several other mechanisms)

Question 129

Cri du Chat is what type of deletion?

Answer 129

Can be seen with routine microscopy or can be small enough to be considered a microdeletion

Question 130

What is duplication?

Answer 130

Duplication – Results in partial trisomy for the duplicated segment

a) Notation: 46,XY,dup(1)(q22q25). The segment of one of the chromosomes 1 has been
duplicated (dup) from q22 to q25.

b) Notation: 46,XY,add(8)(p23). There is a piece of additional (add) chromosomal material
on the short arm of chromosome 8, attached at 8p23, but the origin of the additional material
is not identified yet.

Question 131

Once a duplication is diagnosed, what must be done?

Answer 131

If a duplication (or any structural abnormality) is diagnosed, you must rule out a
rearrangement in one of the patient’s parents

Question 132

What is contiguous gene syndrome?

Answer 132

Usually refers to a phenotype caused by a deletion of several genes, but could also be a duplication of several genes (a microduplication). Since about 1/3 of all our genes relate to brain development and many of the other loci relate to the control of morphogenesis of the embryo, most microdeletions involving several genes will result in a phenotype comprising dysmorphism (abnormal physical features), organ malformations, and intellectual deficit. Many
of these were previously thought to be dominant or recessive syndromes caused by single genes.

Question 133

What are translocations?

Answer 133

Translocations – Relocation of a whole chromosome or portion of a chromosome to another chromosome

Question 134

What is a balanced versus unbalanced translocation? Potential complication effect?

Answer 134

What is most important for the individual to be normal is that the correct amount of genetic material is present (the translocation is balanced –there are neither extra nor missing “pages” – one just has to look in one of the other “books”
to finish reading the “recipe”) and that none of the “recipes” (genes) has been disrupted –
i.e., that all the information remains able to be read, or that portions of two genes have not
been placed next to each other so that they make up a new, deleterious product (position
effect) (e.g., a peanut butter and jelly sandwich recipe translocated with a liver and onions
recipe could result in peanut butter and liver sandwiches…..). If the individual has too
much or too little genetic material, or if a gene has been disrupted so that it cannot be used
properly, the translocation is called unbalanced.

Question 135

Compare outcomes of balanced versus unbalanced translocations

Answer 135

(1) Individuals with unbalanced rearrangements are usually physically and/or intellectually abnormal.

(2) Individuals with balanced rearrangements are phenotypically normal. However, during reproduction they may pass on their translocation in either balanced or unbalanced form – therefore, they have increased risk to have
abnormal offspring.

Question 136

What are reciprocal translocations?

Answer 136

Exchange of genetic material between non-homologous chromosomes (i.e.,
chromosomes from different pairs) or between homologous chromosomes at nonhomologous
sites (much less common).

Question 137

Carriers of balanced reciprocal translocations have an increased risk of?

Answer 137

Carriers of balanced reciprocal translocations have an increased risk to have offspring with partial monosomy for one of the involved chromosomes and/or partial trisomy for the other chromosome.

Question 138

What is robertsonian translocation?

Answer 138

A translocation involving two acrocentric (#13, 14, 15, 21, or 22) chromosomes (may involve homologous chromosomes —e.g., two #13s— or nonhomologous chromosomes —e.g., a #14 and a #21) which have joined at or near the centromere (i.e., the front covers of two books are torn off and the two books are stapled together front-to-front.) The short arm material is lost, but there are no phenotypic consequences of losing this material from acrocentric chromosomes. This is because the acrocentric short arms only code for ribosomal RNA (the nucleolar organizing regions, NOR’s, are in the stalks of the satellites).

Question 139

Risk of robersonian translocation?

Answer 139

The normal, balanced carrier
has a risk of having unbalanced offspring with trisomy or monosomy (those
with monosomy are unlikely to survive past early pregnancy).

Question 140

Describe the balanced carrier of robertsonian translocation

Answer 140

Balanced carrier of a Robertsonian translocation: Notation: 45,XX,der(14;21)(q10; q10). The total number of chromosomes is 45 because
two of them have joined together to form a single, larger chromosome, which was derived (der) from the long arms of chromosomes 14 and 21.

Question 141

Describe the unbalanced carrier of robertsonian translocation

Answer 141

Unbalanced carrier of a Robertsonian translocation: Notation: 46,XX,der(14;21)(q10;q10),+21. This individual has a total of 46 chromosomes, but one of her 14’s has a #21 attached to it. Therefore, this individual has an
extra chromosome 21 (a total of 47 chromosomes’ worth of DNA, but you only
see 46 individual pieces…….).

Question 142

What are insertions?

Answer 142

Insertions – A segment from one chromosome is inserted into another chromosome

Question 143

What are inversions?

Answer 143

Inversions – a piece of chromosome breaks out, turns upside-down, and re-inserts itself in the
same place

Question 144

How does inversion occur?

Answer 144

At meiosis, in order for the inverted chromosome to pair with its homologue along its entire
length, it has to flip over at the inverted part and form a reversed loop (inversion loop).

Question 145

Inverted DNA will lead to embryos with?

Answer 145

The resulting conceptuses (embryos)
would have either a partial trisomy for one distal segment and a partial monosomy for
the other, or vice versa. In general, the one with the least amount of monosomy is the only
one likely to be viable (i.e., the less that’s missing, the better it is…..)

Question 146

What is a pericentric inversion?

Answer 146

Pericentric inversions – the inverted segment includes the centromere. Recombinant
results in partial monosomy and partial trisomy.

Notation: 46,XY,inv(7)(p14.2q36.3).

Question 147

What is a paracentric inversion?

Answer 147

Paracentric inversions – the inversion occurs to one side or the other of the centromere and
does not include it.

Notation: 46,XY,inv(3)(q13q24).

Question 148

What is an isochromosome?

Answer 148

Isochromosome – a “mirror-image” chromosome comprising either two copies of the long arms and no short arms, or vice versa.

a) Normally, chromosomes divide by longitudinal separation at the centromere into two
chromatids. However, if a chromosome undergoes transverse separation at the centromere, the two daughter chromosomes will not be equal but rather will represent a smaller
chromosome (2q’s, no p) and a larger chromosome (2 p’s, no q).

Question 149

What is a ring chromsome?

Answer 149

Results from loss of telomeres from both the short and long arm of a chromosome and fusion of the “sticky ends”. Results in partial monosomy of the end of the short arm and also of the end of the long arm.

Question 150

What is a marker chromosome?

Answer 150

An abnormal, usually smaller, chromosomethat cannot be identified by banding. FISH is
often useful in the characterization of the marker chromosome; array CGH also can be used.

Question 151

What are autosomal fragile sites?

Answer 151

Autosomal fragile sites - not associated with clinical abnormality

Question 152

What is Fragile X?

Answer 152

Fragile X: an abnormality in the distal long arm of the X chromosome (Xq27) due to unstable DNA trinucleotide repeat sequences.

Question 153

What is spontaneous abortion? Frequency?

Answer 153

The term, “spontaneous abortion” (SAb) is used for pregnancy loss (miscarriage) up to 20 weeks’
gestation.

1. The frequency of pregnancy loss is estimated to be from 10-50% of all conceptions,
   depending on the method used to detect the pregnancy,

Question 154

Most common cause of miscarriage?

Answer 154

The most common cause of miscarriage is a chromosome abnormality.

Question 155

Chromosome anomalies account for what amount of miscarriages? When? Percentage that are trisomies?

Answer 155

Chromosome abnormalities account for at least 50% of all SAbs and for ~70% of SAbs occurring in the 1st trimester (up to the 12th week of pregnancy).

50% of the chromosome abnormalities are trisomies

Question 156

Chromosomal anomaly in couples with many miscarriages?

Answer 156

In ~5% of couples who have had ≥3 SAbs, one partner carries a balanced chromosomal
rearrangement (compared with 0.55% of the general population); their risk of chromosomally abnormal offspring in future pregnancies is increased. Therefore, couples with this history should be karyotyped.

Question 157

Describe the Y chromosome. Variation in size?

Answer 157

The Y chromosome is in the same size range as the two smallest pairs of autosomes (#21-22).

It has relatively few genes (59 genes and disorders as of January 2014)

The size of the Y can vary markedly without any clinical effect because there is a variable-length distal segment of the Y long arm that does not contains any genes.

Question 158

Sex determination and the Y chromosome

Answer 158

The Y chromosome (or, more specifically, a gene on the Y chromosome short arm (Yp), is a
dominant determinant for testis development and determines gender in humans (the testis determining factor, TDF), known as SRY (sex-determining region on Y). That is, human
embryos develop as females unless SRY is present and causes the indifferent gonad to develop into a testis.

Question 159

What is the pseudoautosomal region?

Answer 159

Unlike autosomal pairs of chromosomes, the heteromorphic X and Y are not completely homologous. There are two regions of complete homology between the X and Y chromosomes at the distal ends of their short and long arms. The X and Y chromosomes pair and cross over in these regions during prophase I. This appears to
be essential for correct segregation of the sex chromosomes. As a result of this crossing over, female offspring of males can inherit DNA sequences from the Y chromosome distal to the point of exchange and vice versa. Therefore, genetic markers in this region of pairing and exchange between the X and Y segregate
independently of sexual phenotype, and so this region is called the pseudoautosomal region.

Question 160

X genes and sexual differentation?

Answer 160

majority of genes on the X have nothing to do with sexual differentiation.

Question 161

What is the Lyon Hypothesis?

Answer 161

Despite the fact that males have one X and females have two X’s, the sexes really do not differ from each other very much, apart from sexual development and secondary sexual characteristics. The relative similarity of male and female mammals is due to a mechanism of dosage compensation that allows all but one X chromosome in each cell to be almost
entirely turned off (inactivated). (The “almost” is very important – there are some genes on the X that escape inactivation.)

Question 162

Describe why Turner phenotype is not so irregular

Answer 162

Single X is enough

Patients missing an entire X chromosome (i.e., Turner syndrome) or those with an entire extra X chromosome (e.g., XXY or XXX individuals) are not very different overall from normal individuals.

Question 163

Difference between genotypes with variable levels of X

Answer 163

It is those few genes on the X that escape inactivation that cause the differences between an XX individual and an XO or XXX individual, or between an XY and an XXY individual.

Question 164

X inactivation is what type of process?

Answer 164

Epigenetic (non-permanent)

Question 165

What is XIC? XIST?

Answer 165

XIC (for X inactivation center) in the human refers to a region on the X chromosome that isrequired for the initiation of X-inactivation and is invariably present on all X chromosomes that
undergo inactivation, including those with structural rearrangements.

There is a specific gene in that region called XIST (X-inactivation-specific transcript), a complex specialized control locus located in the proximal q arm of the human X chromosome (at Xq13.2) that is the master regulatory switch locus for X-inactivation. XIST is necessary for X inactivation (but alone is not sufficient).

Question 166

How to help the lab?

Answer 166

The more clinical information you give the laboratory, the better analysis and interpretation they can provide.

1. If you tell the lab the specific abnormal clinical features, they can look closely in any regions
   known to cause those abnormalities or suggest other techniques to use.
2. If you are looking for a specific microdeletion or other specific anomaly that requires special
   techniques, you must tell the lab which anomaly or condition you are looking for so they can
   use the proper probe(s).

Question 167

Parental analysis with numerical abnormality?

Answer 167

For patients who have numerical abnormalities, e.g. trisomy, monosomy, or triploidy, chromosome analysis of their parents is not needed because these anomalies arise de novo.

Question 168

Parental analysis with structural abnormality?

Answer 168

For patients who have structural abnormalities, e.g. duplications, deletions, translocations, etc.,
parental karyotype analysis is essential because:

1. One of the parents may have the rearrangement in balanced form
2. Knowing whether the rearrangement in the patient was inherited from a parent or occurred
   de novo will help assess recurrence risk (the chance that they may have another abnormal
   baby) for the parents’ future pregnancies.
3. If the patient’s parent carries a balanced rearrangement, one of his or her parents (i.e., the
   patient’s grandparent) may also carry the balanced rearrangement and may have passed it to others of his/her children (i.e., the patient’s aunts and uncles), who probably are not aware
   that they may be at-risk to have chromosomally abnormal children.

Question 169

What to consider if test is normal, but phenotype is off?

Answer 169

If you suspect a specific chromosome abnormality on the basis of the phenotype of the patient but the blood karyotype, FISH, microarray, etc. are normal, and you are still suspicious, consider the possibility of mosaicism and either examine a much larger number of cells or test another tissue, e.g. skin

Question 170

Two modes of Prader Willi

Answer 170

Deletion of 15q for father

Inheritance of only mom 15s

Question 171

What is a haplotype?

Answer 171

A haplotype (from the Greek: ἁπλοῦς, haploûs, “onefold, single, simple”) in genetics is a combination of alleles (DNA sequences) at adjacent locations (loci) on a chromosome that are inherited together. A haplotype may be one locus, several loci, or an entire chromosome depending on the number of recombination events that have occurred between a given set of loci, if any occurred.

Question 172

What is difference between introns and exons?

Answer 172

Exons are expressed
Introns are not expressed
Splicing

Question 173

What is a locus?

Answer 173

In genetics, a locus (plural loci) is the specific location of a gene or DNA sequence or position on a chromosome

Question 174

Simplex vs sporadic?

Answer 174

“Sporadic” refers to a chance event. “Simplex” refers to a single occurrence of a condition in a family.