CGDpheno1_Protocol
Project
protocol
—
Contents
General
workflow
and
sampling
Procedure:
Blood
chemistry
and
electrolyte
measurement
using
Beckman
CX5
Synchron
Delta
Chemistry
Autoanalyzer
Workflow
and
sampling
Equipment
and
supplies
Reagent
and
solutions
Definitions
and
calculations
Procedure:
Complete
blood
count
(CBC)
with
differential
using
the
Bayer
ADVIA
120
Hematology
Analyzer
Workflow
and
sampling
Equipment
and
supplies
Reagents
and
solutions
Definitions
and
calculations
Procedure:
Bone
mineral
density
and
body
composition
measurement
using
DXA
PIXImus
Workflow
and
sampling
Equipment
and
supplies
Reagents
and
solutions
Definitions
and
calculations
Statistical
analysis
and
calculations:
Mixed-effect
model
fitting
(ANOVA
adjustment)
Data
References
General
Workflow
| Tests |
Age
(wks) |
Equipment
used |
Data
collected |
|
| 11 |
Bayer
ADVIA
120 |
Complete
differential
cell
count |
| Blood
plasma
chemistry
| 10,
12 |
Beckman
CX5
Synchron
Delta |
Complete
plasma
chemistry |
|
| 13 |
DXA
PIXImus |
Fat,
lean,
total
composition;
whole
BMD |
Acclimation
to
test
conditions
In
general
all
mice
are
brought
into
the
procedure
room
and
are
tested
within
1hr.
--------------------------------------------------------------
Blood
Plasma
Chemistry
Workflow
and
sampling
| Steps |
Procedure
accomplished |
Time
used
(hr) |
#
of
Samples |
Data
collected |
1 |
Mice
are
fasted:
food
and
water
removed
for
4h |
0.5 |
- |
- |
2 |
Sample
tubes
prepared
for
blood
collection |
0.5 |
80
samples/batch |
- |
3 |
Blood
collected
via
retro-orbital
vein |
2.5 |
80
samples/batch |
- |
4 |
Post-blood
collection
clean-up |
0.5 |
80
samples/batch |
- |
5 |
Blood
samples
centrifuged
at
4°C |
1.0 |
80
samples/batch |
- |
6 |
Plasma
extracted
(frozen
when
stored) |
1.0 |
80
samples/batch |
- |
7 |
Beckman
CX5
system
calibrated |
0.25 |
- |
- |
8 |
Reagents
changed
or
replenished |
0.25 |
- |
- |
9 |
System
controls
run |
0.25 |
- |
- |
10 |
Plasma
HDL
test
prepared |
2.5 |
15
sectors
(105
samples)/run |
- |
11 |
Plasma
HDL
measured
automatically |
1.0 |
15
sectors
(105
samples)/run |
- |
12 |
Plasma
CHOL,
GLU
and
TG
prepared |
1.0 |
15
sectors
(105
samples)/run |
- |
13 |
Plasma
electrolytes,
lipids,
glucose,
and
proteins
measured
automatically |
3.0 |
15
sectors
(105
samples)/run |
Na,
Cl,
K,
CO2,
CHOL,
GLU,
TG,
HDL,
NEFA,
T4,
TBIL,
BUN |
14 |
Final
clean-up |
0.5 |
- |
- |
15 |
Computer
printed
data
are
labeled,
data
files
collected
and
stored
on
disks |
0.5 |
- |
- |
Equipment
and
supplies
- Refrigerated
tabletop
micro-centrifuge:
Eppendorf
Centrifuge,
Model
#
5415C.
- Repeat
pipettes
and
regular
Pipetman:
250
µL
and
100
µL,
respectively.
- Automated
blood
chemistry
analyzer:
Synchron
CX5
Delta
(Beckman
Coulter,
Inc.,
Fullerton,
CA).
- A
dedicated
DOS-based
desktop
computer
controls
the
programming
of
this
analyzer.
- A
dedicated
printer
prints
the
results
as
they
are
measured,
and
an
electronic
file
is
simultaneously
transferred
to
a
second,
Windows-based
computer,
which
stores
the
data
files.
- Micro-hematocrit
tubes
(75µL
capacity)
coated
with
Heparin
and
equipped
with
a
rubber
bulb
expunger
- Expendables:
(1)
1.5
µL
Eppendorf
tube,
(2)
0.5
mL
Beckman
Coulter
Microtube
Tubecup
("sector
cup")
(3)
100
µL
and
250
µL
pipette
tips
(4)
1
cc
syringes
with
needles
Panels
A-E
illustrate
the
Beckman
Synchron
CX5
Delta.
Panel
B
shows
a
closer
look
of
area
1
in
Figure
A.
Figure
C
presents
a
closer
look
of
area
2
in
Panel
A.
Panel
D
depicts
a
closer
view
of
area
3,
where
ancillary
reagents
are
refilled
in
Panel
A.
Panel
E
reveals
the
content
of
area
4,
where
samples
are
set
up
in
trays
for
an
automated
run
in
Panel
B.
Reagents
and
solutions
- Heparin
anticoagulant
(Sigma
(Sodium
Salt)
50,000
U
Cat.
#H-3393)
->Heparin
1000U/mL:
50mL
of
distilled
autoclaved/sterile
water
+
50,000U
Heparin
Stock
Solution
- Sterile
physiological
(0.9%)
saline
solution
- Reagents:
The
Chemistry
Analyzer
(or
"CX5")
uses
Beckman
Coulter
three-compartment
reagent
cartridges
for
HDL,
CHOL,
TG,
and
GLU.
Each
cartridge
contains
enough
reagents
for
300
tests
(approximately
104
mL).
In
addition,
in
order
to
run
the
HDL
Cholesterol
test,
HDL
Cholesterol
Separation
Reagent
(15
µL
per
sample)
is
needed.
The
bottle
from
Beckman
Coulter
contains
a
volume
of
34
mL.
If
the
dilution
of
plasma
samples
becomes
necessary
due
to
low
plasma
volume,
use
0.9%
saline
solution
for
the
dilution.
- Reagent: Reorder
No.
Cholesterol
(CHOL)
Reagent
467825
Glucose
(GLU)
Reagent
442640
Triglycerides
(TG)
Reagent
445850
- Calibration
Reagents:
The
two
calibration
reagents
are
"Synchron
Systems
HDL
Cholesterol
Calibrator"
(for
HDL
only),
and
"Synchron
Systems
Multi
Calibrator"
(for
CHOL,
GLU,
and
TG).
- Controls:
The
controls
for
HDL
are
Beckman
Coulter
Vigil
Lipid
Control
1
and
Beckman
Coulter
Vigil
Lipid
Control
2.
The
controls
for
CHOL,
GLU
and
TG
are
Synchron
Control
Comprehensive
Chemistry
Control
Serum
Level
1,
Level
2
and
Level
3.
I.
Blood
plasma
collection
a.
Blood
samples
are
obtained
from
each
animal
at
10
and
12
weeks
of
age
(after
4h
fast
from
0700
-
1100
h).
b.
Approximately
200
µL
of
blood
are
obtained
from
mice
via
retro-orbital
bleed
using
heparin-coated
Hematocrit
tubes.
Remaining
blood
in
the
Hematocrit
tube
is
flushed
out
using
a
rubber
squeeze
bulb
assembly.
Investigator's
note:
In
order
to
be
able
to
bleed
the
mice
the
following
week
for
another
test,
the
same
volume
of
blood
taken
is
replaced
subcutaneously
with
sterile
physiological
saline.
c.
Blood
samples
from
12-wk
old
mice
are
collected
into
pre-labeled
1.5
mL
Eppendorf
tubes
pre-loaded
with
7.5
µL
of
the
anticoagulant
Heparin
1000U/mL,
gently
finger
flicked
and
mixed
or
stirred,
and
momentarily
stored
in
ice
until
all
the
samples
are
ready
to
be
centrifuged.
Blood
samples
from
10-wk
old
mice
destined
for
electrolytes
analysis
are
collected
without
pre-loading
with
heparin.
d.
Blood
samples
are
then
centrifuged
for
5
min
at
14,000
RPM
using
a
refrigerated
table-top
micro-centrifuge
to
separate
the
plasma.
e.
The
top
plasma
(for
heparinized
samples,
or
serum
for
non-heparinized
samples)
layer
is
pipetted
(~100µL)
into
pre-labeled
0.5
mL
Eppendorf
tubes
and
frozen
until
ready
to
be
assayed;
remaining
packed
blood
cell
layer
is
discarded.
f.
Previously
frozen
samples
are
defrosted
at
room
temperature
for
about
30
min
before
measurements
are
done.
NOTES:
Air
bubbles
are
avoided
and
eliminated
during
sample
loading
in
sector
cups
as
they
interfere
with
the
colorimetric
assay.
II.
Using
Beckman
CX5
Synchron
system
to
measure
plasma
glucose
and
lipids
chemistries
Panel
F
shows
2
empty
sector
cups.
Panels
G
shows
sector
cups
with/out
hemolyzed
sample,
and
Panel
H
shows
sector
cups
without
and
with
(red
arrow)
air
bubbles.
Panels
I
and
J
show
consecutive
sector
trays
identified
with
bar
codes
and
seven
sector
cups
contained
within
each
tray.
a.
In
preparation
for
the
auto-analyzer,
bar-coded
sectors
with
cups
in
place
are
loaded
with
85
µL
of
completely
thawed
plasma
(enough
for
the
direct
measurement
of
CHOL,
GLU,
and
TG).
b.
Up
to
five
sectors
are
manually
placed
on
the
carousel
to
be
run.
Since
each
sector
is
bar-coded,
the
Beckman
automatically
detects
a
sector
that
has
been
run;
regardless,
finished
sectors
are
removed
immediately
as
soon
as
they
come
up.
c.
The
Beckman
CX5
is
operated
according
to
manufacturer's
instructions
in
the
measurement
of
plasma
HDL,
CHOL,
GLU,
and
TG,
which
are
run
together.
d.
-Function
key
F1
is
used
to
deploy
"Sample
Program",
Sample
type
"2"
is
for
plasma.
-Function
key
F2
is
used
to
deploy
"Program
Batch/Sector(s)"
and
"sector(s)
to
program:"
(i.e.
sectors
1-5
is
programmed).
When
"Batch
mode
activated,
7
cups
possible.
"Number
of
cups
in
batch:"
message
is
displayed,
the
total
cups
for
this
batch
is
then
(7
x
5)
=
35
cups
(the
maximum
number
of
cups
that
can
be
ran
in
a
batch
is
98).
To
program
remaining
sectors,
F2
Program
Batch
is
deployed
again.
-Panel
"12"
is
preprogrammed
for
CHOL/GLU/TG
and
"HDLD"
is
manually
"Selected"
from
the
screen
menu.
Once
the
correct
chemistries
are
selected,
they
are
"ENTERed"
to
bring
about
"SAMPLE
TYPE",
wherein
"2"
is
given
to
denote
plasma
(not
serum).
-Function
key
F8
is
used
to
set
up
the
programmed
batches
and
to
advance
to
the
next
cup/sample
(from
cup
#1
up
to
cup
#7)
in
a
given
sector.
By
selecting
F8
ID
numbers
can
be
recorded
and
reviewed
against
an
Excel
reference
sheet.
Notes:
Since
ID
sample
numbers
or
field
identifiers
are
un-editable
once
Beckman
CX5
is
in
operation,
relevant
information,
including
sample
type
(i.e.
plasma
vs
serum),
dilution
factor,
and
other
information
must
be
precisely
entered.
-
As
soon
as
six
sectors
are
programmed,
the
<prev
screen>
is
activated
first,
and
then
the
Master
Screen,
and
then
last
START
(green)
button.
The
Beckman
automatically
starts
sampling
the
first
five
programmed
sectors.
Additional
sectors
can
be
programmed
while
the
Beckman
is
operating.
-In
the
event
that
the
Beckman
alarm
is
activated
because
of
reagent
volume
getting
low,
<prev
screen>
is
activated
to
turn
off
the
alarm
and
make
the
necessary
notations
for
the
record.
The
next
available
reagent
cartridge
is
automatically
installed.
-When
all
the
data
is
safely
recorded,
Function
key
F5
is
used
to
clear
all
the
information
regarding
a
sector
after
ENTERing
the
number
of
the
sector
to
be
deleted.
e.
Once
a
sector
is
finished
running,
the
results
are
automatically
printed,
removed
from
the
printer,
and
then
labeled
accordingly.
Otherwise,
the
printed
paper
is
checked
and
guarded
from
rolling
back
into
the
printer
and
disrupting
the
data
recording.
f.
Used
Eppendorf
tubes,
pipette
tips,
sector
cups,
and
reagent
cartridges
are
discarded
into
biohazard
waste
containers,
and
any
spilled
liquids
are
cleaned.
For
additional
information
Definition
and
calculation
The
average
of
the
diluents
analyzer
value
is
subtracted
from
the
analyzer
value
multiplied
by
two
(dilution
factor)
to
obtain
the
HDL
(indirect)
values.
HDL
(indirect)
values
=
(sample
analyzer
value
x
2)
-
average
of
diluents
analyzer
value
-----------------------------------------------------------------
Hematology
Workflow
and
sampling
Test |
Procedure
performed |
Volume
(µL)
|
Data
collected |
1 |
Body
weight
measurement
|
- |
body
weights |
2 |
Blood
collection;
samples
are
kept
at
24°C
(for
<3
h)
until
testing
|
200 |
- |
3 |
Hematology
samples
are
run
on
the
ADVIA
120
Hematology
Analyzer |
200 |
Complete
blood
cell
counts
(CBC)
with
differential
|
Equipment
and
supplies
Panel
A
shows
the
Bayer
ADVIA
120
hematology
analyzer
system.
Panel
B
shows
the
internal
layout
of
the
ADVIA,
and
the
various
reagents
used
in
the
system.
Panel
C
shows
the
hematology
setup,
equipped
with
a
computer
and
a
printer.
Panel
D
shows
a
typical
computer
screen-output.
Reagents
and
solutions
Bayer
Diagnostics
(Siemens
Healthcare
Diagnostics)
•
ADVIA
TESTpoint
Hematology
Controls
•
ADVIA
120
autoRETIC
Reagent
T01-3622-01
•
Perox
Sheath
T01-3633-01
•
Perox
1
T01-3630-01
•
Perox
2
T01-3631-01
•
Perox
3
T01-3632-01
•
RBC/PLT
T01-3627-01
•
HGB
T01-3628-01
•
BASO
T01-3629-01
•
AutoRETIC
T01-3622-01
•
EZ
KLEEN
T01-3624-01
•
Defoamer
T01-3625-04
•
Sheath/Rinse
T01-3664-01
- 20%
EDTA,
Tetrasodium
Salt
(Fisher
Lab
item
number
BP121-500),
anticoagulant
Procedure:
Complete
blood
count
(CBC)
with
differential
using
the
Bayer
ADVIA
120
Hematology
Analyzer
Blood
collection
a.
Blood
samples
are
obtained
from
each
animal
at
10
weeks
of
age
(non-fasted).
b.
Collection
tubes
(1.5
mL
Eppendorf)
are
pre-loaded
with
20
µL
of
20%
EDTA.
c.
A
clean
retro-orbital
bleed
is
performed
using
EDTA-coated
microhematocrit
tubes.
d.
Blood
collection
tubes
are
filled
to
a
final
volume
of
200
µL
and
then
kept
at
room
temperature
for
the
duration
of
the
test.
e.
The
blood
sample
is
checked
for
clots
using
a
toothpick.
(In
the
presence
of
a
clot,
the
sample
is
discarded
to
avoid
"aspiration
failure"
and
lost
data
during
sample
run.)
Using
Bayer
ADVIA
120
system
to
conduct
CBC
with
differential
and
reticulocytes
count
a.
Blood
samples
are
gently
mixed
well
(by
rolling
the
vial
the
between
hands)
and
kept
at
ambient
temperature.
b.
Samples
are
run
according
to
manufacturer's
instructions.
c.
As
part
of
ADVIA
daily
routine
maintenance,
a
control
run
is
initially
performed.
This
usually
takes
about
25
min
to
do.
Since
controls
contain
human
blood
cells
in
a
preservative
medium,
proper
safety
precaution
is
exercised
with
the
use
of
disposable
gloves.
d.
As
long
as
calibrated
commercial
controls
are
within
established
ranges,
the
PRIMER
sample
can
be
run
first
(to
get
the
system
"wet")
in
preparation
for
the
test
samples.
Each
run
takes
about
1
min,
when
done
through
open
tube
aspiration
wand.
e.
To
prevent
"aspiration
failure"
or
loosing
a
sample
run,
the
blood
sample
is
double-checked
for
clots
so
that
no
air
gap
is
introduced
while
the
sample
is
being
aspirated.
f.
After
each
successful
run,
a
lab
screen
pops
up
that
can
be
hidden
to
return
to
Manual
Sample
ID
Screen,
and
to
review
the
result
via
the
quality
control
(QC)
button.
g.
After
a
hard
copy
of
a
successful
run
is
automatically
printed,
the
next
sample
is
ready
to
be
run.
h.
Values
reported
are
those
obtained
directly
from
the
ADVIA.
i.
No
correction
for
the
small
dilution
is
made.
j.
For
additional
information.
Definitions
and
calculations
This
figure
illustrates
a
close-up
display
of
the
computer
screen
result
in
Panel
D
above.
WBC
differential
percentages
were
computed
for
each
cell
type
as
follows:
- %
NEUT
=
[(NEUT
count
x
106)
÷
(total
WBC
count
x
106)]
x
100
- %
LYMPH
=
[(LYMPH
count
x
106)
÷
(total
WBC
count
x
106)]
x
100
- %
MONO
=
[(MONO
count
x
106)
÷
(total
WBC
count
x
106)]
x
100
- %
EOS
=
[(EOS
count
x
106)
÷
(total
WBC
count
x
106)]
x
100
- %
BASO
=
[(BASO
count
x
106)
÷
(total
WBC
count
x
106)]
x
100
- HCT
(hematocrit)
=
(RBC
X
MCV)÷10
representing
the
PCV
(packed
cell
volume)
- %
Retic
=
[(Retic
count
x
109)
÷
(total
RBC
count
x
109)]
x
100
--------------------------------------------------------------
Bone
mineral
density
and
body
composition
Workflow
and
sampling
|
|
Age
(wks) |
Equipment/Reagent |
Data
Collected |
|
Obtained
body
weight |
|
|
body
weight |
|
Mice
anesthetized
and
measured
for
body
length |
13 |
needles
and
syringes,
anesthesia
|
body
length |
|
DXA
system
prepared
and
calibrated |
- |
DXA
system |
- |
5 |
Whole
body
scan
|
13 |
DXA
system |
whole
body
scan
images |
|
Analysis
of
whole
body
scan
images |
13 |
DXA
system |
bone
mineral
density
(BMD),
fat
and
lean
tissue
mass |
Equipment
and
supplies
- Top
loading
balance:
Ohaus
Portable
Navigator
Series
Electronic,
Model
NV-210
(Ohaus
Corp.,
Pine
Brook,
NJ)
for
measuring
body
weights.
- DXA
scanning
by
PIXImus:
The
Lunar
PIXImus
small
animal
DXA
system
(PIXImus™,
Fitchburg,
WI)
was
used
to
assess
whole
body
areal
(a)BMD
and
body
composition
at
16
weeks
of
age.
This
methodology
has
been
validated
in
small
animals
(see
Nagy,
2000;
Nagy,
2001).
- Disposable
specimen
trays
with
sticky
immobilizing
tape:
Lunar
PIXImus
Corporation
Headquarters,
726
Heartland
Trail,
Madison,
WI
53717,
Phone:
800-445-8627,
Fax:
608-826-7102.
- Needles
and
syringes
- Mouse
densitometer
dual
energy
X-ray
absorptiometry
(PIXImus
small
animal)
DXA
system
(GE-Lunar,
Madison,
WI):
The
PIXImus
mouse
densitometer
has
been
reconfigured
with
lower
x-ray
energy
than
in
human
DXA
machines
in
order
to
achieve
optimal
contrast
in
small
specimens.
The
Lunar
PIXImus
for
rodents
is
a
fully
integrated
densitometer
designed
for
the
estimation
of
bone
mineral
density
(BMD)
and
body
composition.
The
resolution
of
the
PIXImus
is
0.18
x
0.18
mm
pixels
with
a
usable
scanning
area
of
80
x
65
mm,
allowing
for
measurement
of
a
single
mouse
or
collections
of
isolated
specimens.
The
PIXImus
has
been
calibrated
with
a
phantom
utilizing
known
values,
and
QA
is
performed
daily
with
this
same
phantom.
The
precision
for
BMD
is
less
than
1%
coefficients
of
variations
(CV)
for
whole
body,
approximately
1.5%
CV
for
specialized
regions
(Nagy
et
al,
2000).
Correlation
with
pQCT
values
for
614
isolated
spinal
vertebrae
is
significant
(p<0.001;
r=.704).
Assessment
of
accuracy
for
the
PIXImus
is
done
with
a
set
of
hydroxyapatite
standards
(0-2,000
mg),
yielding
a
correlation
of
0.999
between
standards
and
PIXImus
measurement
of
mineral.
Full
body
scans
and
X-ray
absorptiometry
data
are
processed
with
manufacturer
supplied
software
(Lunar
PIXImus
2,vers.
2.1).
For
additional
information:
http://piximus.com/
Figure
1
A:
Lunar
PIXImus2
densitometer
with
integrated
PC
computer.
Figure1
B:
Close-up
detail
of
the
densitometer
with
specimen
tray.
Reagents
and
solutions
- Freshly
prepared
solution
of
tribromoethanol
for
anesthesia
- Cleaning
supplies
and
disinfectant
Procedures:
Bone
mineral
density
and
body
composition
measurement
using
DXA
PIXImus
I.
Collecting
image
scans
PIXImus
(small
animal
DXA
system,
PIXImus™,
Fitchburg,
WI)
scanning
of
mice
for
BMC
and
body
composition
is
both
accurate
and
precise
although
body
size
must
be
considered
when
comparing
inbred
strains.
Full
body
scans
are
obtained
and
X-ray
absorptiometry
data
gathered
and
processed
with
manufacturer
supplied
software
(version
1.43.036.008).
a.
The
PIXImus
densitometer
apparatus
is
initially
calibrated
with
a
"phantom
mouse"
according
to
manufacturer's
protocol.
b.
13-wk
old
mice
are
first
weighed
and
body
weight
recorded,
anesthetized
intraperitoneally
with
tribromoethanol
at
a
dose
of
0.2
mL/10g
body
weight,
and
then
measured
for
body
length
(from
the
tip
of
the
nose
to
the
base
of
the
tail).
c.
Fully
anesthetized
mice
are
positioned
dorso-ventral
with
the
tail
positioned
away
or
alongside
from
the
body,
the
front
legs
extended
to
the
side,
and
the
neck
and
spine
are
gently
straightened.
d.
Then
each
mouse
is
placed
on
the
specimen
sticky
tray
(body
must
be
within
blue
line
on
the
tray)
under
the
PIXImus
beam
path
(see
Figure
1B
above).
The
tail
is
placed
alongside
the
body,
the
front
legs
are
extended
to
the
side,
and
the
neck
and
spine
are
gently
straightened.
e.
Trays
are
positioned
such
that
the
area
of
the
head
is
always
oriented
toward
the
left
from
the
investigator's
point
of
view,
and
the
mice
are
position
dorso-ventral-
in
order
to
scan
the
entire
body
and
tail.
The
X-ray
process
to
obtain
a
single
full
scan
is
approximately
5
minutes;
data
can
be
manipulated
subsequently
to
obtain
specific
regions
of
interest
(ROI's).
f.
After
the
whole
body
(excluding
the
head)
is
scanned,
the
isolated
head
alone
is
also
scanned.
g.
Disposable
plastic
trays,
with
sticky
tape
for
immobilizing
mice,
can
be
saved
and
re-used
after
a
thorough
cleaning
and
disinfections.
Investigator's
notes:
To
accommodate
the
large
scope
of
this
project,
animals
are
phenotyped
in
“rounds”
beginning
every
three
weeks,
over
a
period
of
approximately
18
mo.
Every
effort
is
made
to
include
a
complete
strain
set
within
each
round.
To
correct
for
seasonal
effects,
changes
in
the
equipment,
and
differences
between
different
mouse
rooms
(A
vs.
B),
C57BL/6J
males
and
females
are
included
in
each
round
for
each
room.
See
CGDpheno2
for
C57BL/6J
controls
over
time.
II.
Measurement
acquisition
and
image
scan
analysis
Based
on
PIXImus
validation
studies
(Nagy,
2000;
Johnston,
2005)
DXA-
estimated
measurements
of
fat
tissue
correlate
well
with
measurements
obtained
from
chemical
extraction.
This
is
made
possible
by
developing
software
versions
with
equations
that
adequately
correct
raw
DXA-estimated
measurements.
a.
Following
the
completion
of
an
image
scan
the
DXA
system
automatically
implements
specialized
software
to
identify
bone
tissue
from
either
fat
tissue
or
from
lean
tissue
based
on
the
resulting
X-ray
densities
at
two
distinct
energy
levels
(Pietrobelli,
1996;
Johnston,
2005).
b.
Visually,
following
the
completion
of
a
scan,
the
mouse
sample
is
then
outlined
with
red
and
green
colored
circle
and
square
to
define
specific
regions
of
interests
(ROIs).
d.
By
using
the
screen
interactive
display,
F3
is
first
clicked
to
prompt
measurement
adjustments,
and
then
clicked
again
for
the
second
time
to
adjust
ROI
(region
of
interest).
e.
The
area
to
be
analyzed
is
defined
(red
box),
and
areas
to
be
excluded
from
the
calculations
are
defined
(green).
The
arrow
keys
are
used
to
adjust
to
the
desired
size,
in
addition
to
holding
the
control
key
down
to
enlarge
or
elongate
the
circle
or
square
areas.
f.
Once
the
desired
ROI
is
achieved,
the
Enter
key
is
clicked
and
resulting
data
measurement
is
displayed.
By
pressing
F5
a
hard
copy
of
the
image
and
the
scan
analysis
result
is
printed.
g.
To
prompt
the
computer
to
finish
the
session,
F8
or
Esc
key
is
clicked
once,
and
then
clicked
again
to
return
to
the
main
menu
screen
where
the
next
subject
to
be
tested
begin.
h.
Acquired
data
is
saved
on
the
hard
drive
and
on
a
zip
or
CD
disk
for
later
archiving.
Safety
For
safety,
gloves
must
be
worn
and
radiation
safety
guidelines
are
strictly
adhered
to,
such
that
technicians
must
be
6
feet
away
from
the
PIXImus
machine
during
scanning.
Definitions
and
calculations
ROI
=
Region
of
interest
Bone
area
measurement
is
generated
by
outlining
or
specifying
the
limits
or
dimensions
of
the
entire
skeletal
bone
regions
of
the
body
(yellow
outline
in
figure
below),
excluding
the
head
(green),
as
regions
of
interest
(ROI,
red)
following
a
full
body
X-ray
scan.
Bone
mineral
content
(BMC)
is
generated
from
PIXImus
density
scans
which
are
assessed
for
accuracy
using
a
set
of
0.0
mg
to
2,000
mg
of
hydroxyapatite
standards.
According
to
the
DXA
system,
bone
mineral
content
(measured
as
the
attenuation
of
the
X-ray
by
the
bones
being
scanned)
is
divided
by
the
area
(also
measured
by
the
machine)
of
the
site
being
scanned
to
obtain
bone
mineral
density
(BMD):
BMC
=
Bone
mineral
content
(g)
BMD
=
Bone
mineral
density
=
BMC
÷
Area
(g/cm2)
Fat
tissue
mass
=
all
tissues
with
low
density
(x-ray
scan)
Lean
tissue
mass
=
Total
body
tissue
mass
-
Fat
tissue
mass
%
Fat
=
(Fat
tissue
mass
÷
Total
body
tissue
mass
)
x
100
--------------------------------------------------------------
Statistical
analysis
and
calculations:
Mixed-effect
model
fitting
(ANOVA
adjustment)
Mixed-effect
model
fitting
(ANOVA
adjustment)
Phenotypes
were
measured
over
an
18-month
period.
Each
round
may
reveal
different
seasonal
or
machinery
effects.
To
adjust
the
round
effect,
a
mixed-effect
model
was
implemented.
Different
room
environments
(room
A
vs
B)
can
also
cause
measurement
variance.
However
the
number
of
strains
measured
in
each
room
at
each
round
is
not
large
enough;
therefore,
only
the
round
effect
is
corrected
for.
In
this
mixed-effect
model,
phenotype
is
explained
by
sex
and
strain
effect
(fitted
terms),
and
by
round
effect
(random
term).
After
the
initial
mixed
model
fitting,
observations
outside
of
1.5*IQR
(interquantile
range)
were
removed.
The
mixed
model
was
refit
and
the
mean
estimators
and
standard
error
(SE)
were
computed.
Data
collected
by
investigators
- blood
—
clinical
chemistry
- total
bilirubin
(plasma
TBIL)
- chloride
(plasma
Cl)
- potassium
(plasma
K)
- sodium
(plasma
Na)
- dissolved-ionized
carbon
dioxide
(CO2)
- glucose
(plasma
GLU,
4h
fast)
- blood
urea
nitrogen
(BUN)
- blood
—
hematology
—
cell
counts
- red
blood
cell
count
(RBC;
per
volume
x
106)
- white
blood
cell
count
(WBC;
per
volume
x
103)
- eosinophil
differential
(percent
of
total
WBC)
- lymphocyte
differential
(percent
of
total
WBC)
- monocyte
differential
(percent
of
total
WBC)
- neutrophil
differential
(percent
of
total
WBC)
- platelet
count
(PLT;
units
per
volume
x
103)
- reticulocyte
differential
(percent
of
total
RBC)
- blood
—
hematology
—
erythrocyte
parameters
- RBC
corpuscular
distribution
width
(RDW)
- mean
RBC
corpuscular
volume
(MCV)
- hemoglobin
concentration
distribution
width
(HDW)
- mean
RBC
corpuscular
hemoglobin
content
(MCH)
- mean
RBC
corpuscular
hemoglobin
concentration
(MCHC)
- hematocrit
(HCT)
- measured
hemoglobin
(HGB)
- mean
platelet
volume
(MPV)
- blood
—
lipids
- HDL
cholesterol
(plasma
HDL)
- total
cholesterol
(plasma
CHOL)
- non-esterified
free
fatty
acids
(plasma
NEFA,
FFA)
- triglycerides
(plasma
TG)
- body
composition
without
head
- percent
fat
- calculated
lean
tissue
mass
- calculated
total
tissue
mass
- body
length
(tip
of
nose
to
base
of
tail)
- body
weight
- whole
body
bone
mineral
density
- thyroxine
(plasma
T4)
|
Test age:
10-13wks