Technical
Article
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Interpretation of biological
and mechanical variations between the Lowry versus Bradford method
for protein quantification
Tzong-Shi Lu, PhD.1*,
Szu-Yu Yiao, BS.1*,
Kenneth Lim, MD.1,
Roderick V. Jensen, PhD.2,
Li-Li Hsiao, MD., Ph.D.1
1Department
of Medicine, Renal division, Brigham and Women’s Hospital, Harvard Medical
School,
Boston, MA; 2Department of Biological Sciences, Virginia Tech,
Blacksburg, VA,
USA.
Citation:
Lu T-S, Yiao S-Y,
Lim K, Jensen RV, Hsiao
L-L. Interpretation of biological and mechanical variations between the
Lowry versus Bradford method for protein quantification.
North
Am J Med Sci
2010; 2:
325-328.
Doi:
10.4297/najms.2010.2325
Availability:
www.najms.org
ISSN:
1947 – 2714
Abstract
Background:
The identification
of differences in protein expression resulting from methodical variations is
an essential component to the interpretation of true, biologically
significant results. Aims:
We used the Lowry and Bradford methods- two most commonly used methods
for protein quantification, to assess whether differential protein
expressions are a result of true biological or methodical variations.
Material & Methods: Differential
protein expression patterns was assessed by western blot following protein
quantification by the Lowry and Bradford methods.
Results:
We have observed significant variations in protein concentrations
following assessment with the Lowry versus Bradford methods, using identical
samples. Greater variations in protein concentration readings were observed
over time and in samples with higher concentrations, with the Bradford
method. Identical samples quantified using both methods yielded
significantly different expression patterns on Western blot.
Conclusions:
We show for the first time that methodical variations observed in these
protein assay techniques, can potentially translate into differential
protein expression patterns, that can be falsely taken to be biologically
significant. Our study therefore highlights the pivotal need to carefully
consider methodical approaches to protein quantification in techniques that
report quantitative differences.
Keywords: Protein assay, protein quantification, Lowry method. Bradford method
Correspondence to:
Li-Li Hsiao, MD., PhD.
65 Landsdowne Street, Rm321, Cambridge, MA 02139, USA. Tel.: (617) 768 8337,
Fax: (617)768 8251, Email: lhsiao@partners.org
*Tzong-Shi
Lu and Szu-Yu Yiao provide equal contribution and share first authorship.
Introduction
Protein
quantification is
an
essential component in
many biological studies, particularly those evaluating
quantitative protein
expression.
However, studies
scrutinizing these techniques are limited and variations resulting from
different methodologies have largely been unreported. This raises the
fundamental question of whether differential protein expressions reported
are a result of true
biological or methodical variations
[1, 2].
Many
diverse absorbance based colorimetric protein assays have been developed
in an attempt to
increase sensitivity and accuracy
[3].
The
Lowry and Bradford methods are the most widely used dye-binding chromogenic
protein assays
[4]. The Bradford assay
is based on the association of specific amino acid residues, arginine,
lysine, and histidine, with
non-conjugated groups of
Coomassie brilliant blue G-250 dye (CBB) in an acidic environment [5].
The bindings
of proteins with CBB result in a color change
leading to a spectral
shift from 465 nm to 610 nm, and the blue color from the CBB–protein complex
is generally measured at 595 nm for its maximal yield. However, variations
resulting from the Bradford method may be due to
1) amino acid composition of each target protein, i.e. percentage of
arginine in the target protein; 2) sample concentrations beyond 100μg/ml -
1000μg/ml [6]; and
3)
pH of buffers or
types of detergents
used.
The
Lowry method [7]
is a colorimetric assay based on the
interaction of protein
with an alkaline copper tartrate solution and Folin reagent. The color is
generated by two steps: 1) formation of protein and copper complex in an
alkaline buffer, and 2) reduction
reaction of Folin
reagent
causing a spectral shift
from 405 nm to 750 nm, with maximal yield at 750 nm.
Ethylenediaminetetraacetic acid (EDTA)
can interfere with
chromophore production
with the Lowry method.
In
this study, we used the Lowry and Bradford methods – two most commonly used
methods for protein quantification, to assess whether differential protein
expressions are a result of true biological or methodical variations.
Materials and Methods
Protein assay
We
quantified protein concentration by either the Bradford or Lowry methods.
Bradford method (Bio-Rad
Protein Assay; cat no. 500-0006) and Lowry method (Bio-Rad DC Protein Assay;
cat no. 500-0116)
were used in this study.
The measurements
were carried out according to the manufactures instructions
(Bio-Rad, Hercules, CA).
Human umbilical vein endothelial cell (HUVEC) cultures
Commercially available human umbilical vein endothelial cells (HUVECs) were
obtained from Lonza (cat no. cc-2517; Allendale, NJ, USA).
HUVECs were cultured in 5% CO2/37ºC incubator and grown in
microvascular endothelial cell growth medium-2 (EGM-2 MV Bullet kit,
CC-3202, Lonza, Allendale, NJ, USA).
HUVECs were grown
to 80% confluence before commencing heat shock treatment (H) to assess the
inducible protein HSP72. Heat shock treatment was performed as previously
described [8]. Briefly, cells were placed into a pre-heated incubator at a
temperature of 43ºC for 30 minutes. Cells were harvested 24 hours following
heat shock treatment. Non-heat shock treated HUVECs (NH) at the same
confluency were used as a control.
Antibodies and reagents
β-actin,
heat shock protein 72
(HSP72)
and albumin were our
target proteins
for this study. For western blot:
Actin (cat no. MAB1501; Millipore, MA, USA) was used at a concentration of
1:5000;
HSP72 antibody (cat no. SPA810;
AssayDesigns,
Michigan, USA) was used at a concentration of 1:1000.
Albumin is commonly used as standard for protein measurements
(cat no. B4287; Sigma, St. Louis, MO, USA).
SDS-PAGE Gel Electrophoresis and Western Blot
Sample media was mixed with 4X loading (sample) buffer containing 5%
b-mercaptoethanol
(Sigma, MO, USA) and Radio-Immuno Precipitation Assay (RIPA) buffer, pH 7.4
(cat no. BP-115, Boston BioProducts, MA, USA).
The samples were then heated for 5 minutes at 95°C.
10-30mg
of sample was loaded onto SDS-PAGE, NuPAGE Bis-Tris pre-cast polyacrylamide
gels using the mini-cell system (Invitrogen, CA, USA).
NuPAGE MOPS SDS running buffer
was used.
500µl of antioxidant was added to the running buffer. Electrophoresis was
performed at 140V-200V until adequate spread of the protein molecular marker
was achieved.
Following SDS-PAGE gel electrophoresis, proteins were then transferred onto
polyvinylidene difluoride (PVDF) membrane (Millipore, MA, USA).
Transfer was achieved using a wet-blot (Bio-Rad) transfer
system.
Standard Towbin transfer buffer was used
containing 25mM Tris, pH 8.3, 192 mM glycine, 20% (v/v) methanol.
Proteins were then visualized with an enhanced chemiluminescence detection
system.
Results
Stability of the Bradford versus Lowry methods
We
first assessed the stability of Bradford and Lowry methods using Albumin.
Serial dilutions were made (0µg/ml, 2µg/ml, 4µg/ml, 6µg/ml, 8µg/ml and
10µg/ml), in triplicates; the measurements were carried out using a time
course of 30 minutes with 5 minutes intervals. Absorbance change was
calculated using the reference point of 0µg/ml at time 0, with all other
samples compared to this; this value was denoted Delta. Samples measured by
the Lowry method remained steady with time at all concentration preparations
with Delta<0.01; while those measured by the Bradford method showed
increasing Delta with time and serial concentrations. Increasing
concentrations were associated with increasing Delta, from 0 to 30 minutes
(2µg/ml: 0.007-0.013; 4µg/ml: 0.004-0.002; 6µg/ml: 0.012-0.04, 8µg/ml:
0.008-0.052; and 10µg/ml: 0.008-0.061) (Figure
1A). We then assessed if these differences in Delta translated into
significantly different protein concentrations. As shown in Figure 1B, there
is a greater variation of readings over time, with each serial dilution with
the Bradford method. Therefore, we have found that the Lowry method yielded
consistent absorbance readings over time with each serial dilution, while
the Bradford method showed unstable results using identical preparations.
Differential protein expression patterns using Bradford and Lowry methods
Our next goal was to assess whether the differential readings observed with
the Lowry and Bradford methods reflected their measurable differential
expression patterns, reported using protein-based techniques. Total proteins
from identical samples were used with the Lowry and Bradford method.
Differential protein expression patterns were assessed using HSP72 on a
background of
β-actin
as our internal control, in human umbilical vein endothelial cells (HUVECs).
β-actin is an abundant
cytoskeletal protein in all cells and is the most commonly used
internal control protein;
HSP72 is universally
induced in all organisms by
stress (8).
Non-heat shock treated (NH) and heat-shock treated (H) cells were subjected
to western blot analysis. Protein lysates were taken from a single source
from each group. For each sample, protein quantification was performed using
both Lowry and Bradford methods in triplicates, followed by western blot
analysis on three separate occasions.
Protein
quantification results demonstrated observable variations with the Bradford
method compared with the Lowry method for each sample. This confirms our
observations in Figure 1 (Fig.
2A).
The coefficient of variation (CV) in individual sample ranges from 0.029 to
0.09 in Lowry while 0.185 to 0.29 in Bradford.
Western
blot analysis of identical samples demonstrated consistent results with
those assessed by the Lowry method compared with the Bradford method
(Fig.
2B). In addition, our results suggest that the variations in protein
expression patterns observed are not due to mechanical error concluded by
the analysis of all samples on three separate occasions.
Fig. 1 The
protein concentration measurements using Lowry is more consistent than
Bradford methods. The albumin, commonly used as standard for protein
measurements, are prepared
in
serial dilutions (0µg/ml, 2µg/ml, 4µg/ml, 6µg/ml, 8µg/ml and 10µg/ml), in
triplicates. The measurements were carried out using a time course of 30
minutes with 5 minutes intervals. (A) Absorbance change was calculated using
the reference point of 0µg/ml at time 0, with all other samples compared to
this; this value was denoted Delta. Delta is < 0.01 at every sample
preparation using Lowry method; while the Delta is increasing in using
Bradford method (2µg/ml: 0.007-0.013; 4µg/ml: 0.004-0.002; 6µg/ml:
0.012-0.04, 8µg/ml: 0.008-0.052; and 10µg/ml: 0.008-0.061).
The X-axis in
figure 1A represents
30-minutes time course on serial
sample preparations;
Lowry
method (solid line) and
Bradford
method (dotted line). The
Y-axis
represents the Delta.
(B)
The Y-axis in figure 1B is protein concentration expressed in logarithmic
10. L: Lowry Method; B: Bradford Method.
Fig. 2
The
protein concentration measurements using Lowry and Bradford resulted in
protein differential expression.
Total proteins are obtained from
cell lysates of untreated HUVEC (NH)
or 6 hours after heat shock treated HUVEC (H1-H3)
from a single source from each group.
(A) Protein concentrations
from identical samples are measured using either Lowry or Bradford method.
The
measurements of protein concentration on all samples show more consistent
using Lowry method while highly variable in Bradford method.
The X-axis in
figure 2A represents
each sample;
I,
II, and III indicate each experiment.
The Y-axis
represents the
protein concentration expressed in logarithmic 10. (B)
The
expression patterns of
Heat
shock protein 72 (HSP72) and
β-actin
from
each group are examined
using Western Blot.
Identical samples show differential expression patterns on Western blot when
concentration measurements are performed using Lowry vs. Bradford methods
(triplicates) (upper
panel). Protein expressions
from Western blots are quantitated using
Image J program
(lower panel). The Y-axis represents
protein expression level.
The X-axis represents the method used for protein concentration
measurements. ANOVA is
used with P < 0.01 (**).
Discussion
In
this paper, we highlight the importance of carefully considering
methodologies used for protein quantification which can potentially yield
false biologically significant results. We show for the first time that
methodical variations observed in these protein assay techniques, can
potentially translate into differential protein expression patterns that can
be falsely taken to be biologically significant. Current literature using
protein-based techniques rarely report methods used for protein
quantification and our study underlines the need to report this information
to allow for accurate data interpretation.
Our data
suggests that
(1) the Bradford method results in greater variations in protein
concentrations with time and in a random fashion; the differences are more
profound in samples with higher concentrations; (2) using
identical
protein samples, Lowry and Bradford methods yield different concentration
readings, subsequently leading to different expression patterns on Western
blots.
No
significant differences
in the
expression patterns of β-actin were detected between the Lowry and Bradford
methods. This may be due to its high abundance in the cell and therefore
variations in its expression may not be significantly detected. However, we
show that methodologies
chosen
for protein
quantification become significantly important particularly when
low abundant proteins are the interest of
study. Therefore, we caution
the use of
β-actin in isolation as an internal control for equal electrophoretic gel
loading to interpret differential expressions of a target protein without
considering methodologies used in protein quantification.
Unfortunately, methods used for protein quantification are commonly chosen
based on individual preferences rather than taking in consideration the
composition of the target protein, sample concentrations,
pH of buffers or
types of detergents
used.
As mentioned above, the
Bradford assay is based on the association of specific amino acid residues,
arginine, lysine, and histidine, while the Lowry method is a colorimetric
assay based on the
interaction of protein
with an alkaline copper tartrate solution and Folin reagent.
We
suggest that when selecting a particular technique for protein
quantification, the target protein’s composition and buffers should be taken
into account.
Acknowledgement
The
funding support of completion of this work is in part provided by SDSC
global foundation.
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