Original Article
Thermal Stability as a Determinant of AAV
Serotype Identity
Antonette Bennett,1 Saajan Patel,1 Mario Mietzsch,1 Ariana Jose,1 Bridget Lins-Austin,1,3 Jennifer C. Yu,1

Brian Bothner,2 Robert McKenna,1 and Mavis Agbandje-McKenna1

1Department of Biochemistry and Molecular Biology, Center for Structural Biology, The McKnight Brain Institute, College of Medicine, University of Florida, Gainesville,

FL 32610, USA; 2Department of Chemistry and Biochemistry, Montana State University, Bozeman, MT 59715, USA
Currently, there are over 150 ongoing clinical trials utilizing
adeno-associated viruses (AAVs) to target various genetic dis-
eases, including hemophilia (AAV2 and AAV8), congenital
heart failure (AAV1 and AAV6), cystic fibrosis (AAV2), rheu-
matoid arthritis (AAV2), and Batten disease (AAVrh.10).
Prior to patient administration, AAV vectors must have their
serotype, concentration, purity, and stability confirmed.
Here, we report the application of differential scanning fluo-
rimetry (DSF) as a good manufacturing practice (GMP)
capable of determining the melting temperature (Tm) for
AAV serotype identification. This is a simple, rapid, cost
effective, and robust method utilizing small amounts of puri-
fied AAV capsids (�25 mL of �1011 particles). AAV1-9 and
AAVrh.10 exhibit specific Tms in buffer formulations
commonly used in clinical trials. Notably, AAV2 and AAV3,
which are the least stable, have varied Tms, whereas AAV5,
the most stable, has a narrow Tm range in the different buffers,
respectively. Vector stability was dictated by VP3 only, specif-
ically, the ratio of basic/acidic amino acids, and was indepen-
dent of VP1 and VP2 content or the genome packaged.
Furthermore, stability of recombinant AAVs differing by a
single basic or acidic amino acid residue are distinguishable.
Hence, AAVDSF profiles can serve as a robust method for sero-
type identification of clinical vectors.
Received 12 March 2017; accepted 18 July 2017;
http://dx.doi.org/10.1016/j.omtm.2017.07.003.
3Present address: Division of Viral Products, CBER/FDA, Silver Spring, MD 20993,
USA

Correspondence: Mavis Agbandje-McKenna, Department of Biochemistry and
Molecular Biology, Center for Structural Biology, The McKnight Brain Institute,
College of Medicine, University of Florida, Gainesville, FL 32610, USA.
E-mail: mckenna@ufl.edu
INTRODUCTION
Adeno-associated viruses (AAVs) are small, �260 Å, T = 1, icosahe-
dral non-enveloped viruses belonging to the Dependoparvovirus
genus of the Parvoviridae family. Their capsids serve as vehicles
to deliver viral-packaged genomes to the nucleus for replication.
Currently, 13 human and non-human primate AAV serotypes and
over 150 genotypes have been identified.1 The AAV capsid is
composed of 60 copies in total of viral protein (VP)1 (�87 kDa),
VP2 (�73 kDa), and VP3 (�61 kDa) in a population ratio of
1:1:10, respectively.2,3 The AAV VPs share a common VP3 C-termi-
nal sequence, with VP1 and VP2 extended at their N-termini. The
VP1 is further N-terminally extended compared to VP2, with the
VP1 unique (VP1u) region containing a phospholipase A2 (PLA2)
domain, required for infectivity.4,5 Differences in amino acid
sequence and capsid structure mediate the interaction of the AAV se-
rotypes with different host cell receptors, leading to alternative cell or
Molecular Therapy: Methods & Clini
This is an open access article under the CC BY-NC-
tissue tropisms. For example, AAV1 has tropism for skeletal muscle,
whereas AAV8 has tropism for the liver (reviewed by Hastie et al.6).

AAV gene therapy has developed into one of the lead treatment
strategies for various monogenetic diseases. These vectors are recom-
binant AAVs (rAAVs), with a transgene expression cassette packaged
instead of the wild-type (WT) viral genome.7 Early development of
the AAV gene therapy system was mostly focused on AAV2.8 How-
ever, novel AAV serotypes have been isolated, along with the discov-
ery that some of these viruses exhibit higher transduction efficiencies
in certain cells or tissues compared to AAV2. This led to a larger
repertoire of available capsids for packaging different therapeutic
genes.9,10 Thus, many recent clinical trials have utilized a range of
AAV serotypes for therapeutic gene delivery.11–13 Significantly, a
rAAV1 vector for treating lipoprotein lipase deficiency is the first
approved human gene therapy biologic and was certified by the Euro-
pean Medical Agency.12

The AAVs share high amino acid sequence identity, resulting in a
need to develop methods for confirming the serotype in clinical grade
vectors prior to administration. However, in contrast to WT AAV
packaging unique genomes, the identity of purified rAAV capsids
cannot be determined by PCR-based sequencing methods. Further-
more, although mouse monoclonal antibodies are available for
some of the AAV serotypes, which can identify their capsids, this is
not the case for all available AAVs.14–17 The engineering of AAVs
for various reasons, including escape from pre-existing neutralizing
host antibodies or improved tissue targeting, which modifies anti-
genic regions, compounds this problem. An alternative for capsid
identification of purified rAAV preparation is mass spectrometry.18

This method has several advantages, including small sample size
(�0.5–5 mg), a low percentage of unique peptide coverage for identi-
fication, and single residue variations that can be detected when
cal Development Vol. 6 September 2017 ª 2017 The Author(s). 171
ND license (http://creativecommons.org/licenses/by-nc-nd/4.0/).

http://dx.doi.org/10.1016/j.omtm.2017.07.003
mailto:mckenna@ufl.edu
http://crossmark.crossref.org/dialog/?doi=10.1016/j.omtm.2017.07.003&domain=pdf
http://creativecommons.org/licenses/by-nc-nd/4.0/


Molecular Therapy: Methods & Clinical Development
compared to theWTAAV sequence. However, disadvantages include
the requirement for serotype-specific proteases, manual manipulation
of the sample, and time required to prepare and analyze the sample.
This includes running a denatured gel, peptide digest, mass analysis,
and database search.18 Thus, there is a need for new or improved
methods for rAAV serotype identification.

Here, we report the application of differential scanning fluorimetry
(DSF), capable of accurate melting temperature (Tm) determination,
for AAV serotype identification. This approach was developed
and applied to the characterization of AAV capsid stability
as previously described.35 This is a simple, cost effective, rapid, and
robust method utilizing small amounts of purified rAAV capsids
(�1011 particles) and a dye (SYPRO Orange). This study analyzed
AAV1–AAV9 and AAVrh.10, where AAV3 refers specifically to
AAV3b. The AAV serotypes displayed specific capsid stabilities in
buffers commonly used for their formulation and storage, with a sin-
gle amino acid difference being detectable. The Tm is dictated by the
VP3 sequence alone, and not VP1, VP2, or the packaged genome,
making it an ideal method for clinical sample authentication.

RESULTS
Stability of rAAV1–rAAV9 and rAAVrh.10 in PBS Buffer Shows

Disparate Profiles

The stability of rAAV1–rAAV9 and rAAVrh.10 in PBS, the most
commonly utilized AAV formulation and storage buffer, was
analyzed using DSF. The AAV samples were produced using the
Baculovirus/Spodoptera Frugiperda 9 (Sf9) cell expression system
or in HEK293 cells, and purified by AVB affinity column chroma-
tography, with genome-containing (full) and empty capsids separated
by sucrose sedimentation gradient, as previously described.19–21 Sam-
ple purity and capsid integrity were confirmed by SDS-PAGE and
negative-stain electron microscopy (EM), respectively (Figure 1A).
The Tm for the purified full and empty capsids, diluted into PBS
buffer, was determined by DSF,22 as described in Materials and
Methods. The Tm is the temperature at which 50% of the sample is
unfolded and bound with dye. The thermal profiles show Tms ranging
from 66.5�C to 89.5�C ± 0.5�C, with rAAV2 being the least stable and
rAAV5 being the most stable, respectively (Figure 1B; Table 1). The
Tm of each AAV was unique, with the exception of AAV7, rAAV9,
and rAAVrh.10 at 77.0�C ± 0.1�C–0.8�C, which could not be distin-
guished within experimental error (Figure 1B; Table 1). Significantly,
the full and empty capsid Tms were similar for all the AAVs tested
(Table 1).

Comparative Stability Analysis of rAAV1–rAAV9 and rAAVrh.10 in

Commonly Used Formulation and Storage Buffers Reveals

Serotype-Specific Stabilities

The observation that rAAV9 and rAAVrh.10 exhibited experimen-
tally the same Tm in PBS buffer, and the knowledge that the compo-
sition, ionic strength, and pH of a buffer could have an impact on
Tm led to further investigation of thermal stability profiles in other
commonly used AAV formulation and storage buffers (Table 1).
The stability of purified full and empty capsids for rAAV1–AAV9
172 Molecular Therapy: Methods & Clinical Development Vol. 6 Septem
and rAAVrh.10, diluted 10x into five additional (to PBS) common
buffers and universal buffer (UB), developed to be insensitive to
pH changes during thermal melting experiments,23 was tested. The
Tms for each AAV in the buffers aligned into three groups:
group I was AAVs with Tms varying by �15�C–20�C, AAV2 and
AAV3; group II was AAVs with Tms varying by �3�C–6�C,
AAV1, AAV4, AAV6, AAV7, AAV8, and AAVrh.10; and group
III was AAVs with Tms varying by <2.0�C, AAV5 and AAV9 (Fig-
ures 2A–2J; Table 1). Comparative analysis of the AAVs in the
different buffers showed that each buffer had a different effect on
each serotype, i.e., no buffer caused a consistent stabilization or
destabilization of all ten viruses tested (Figure 2K; Table 1). Of
note, only minor Tm fluctuations, �1�C–2�C, were observed be-
tween full and empty capsids of a few AAVs, whereas most showed
no detectable Tm difference (Figure 3; Table 1). For Tms showing mi-
nor differences, there was no trend of full or empty capsids being
more or less stable.

Small Volume and Low Concentration Requirement of AAV

Samples for DSF Analysis

An important aspect of developing DSF profiling as a method for
determining capsid stability and serotype identity was to determine
the minimal amount of AAV required for the assay. Thus, purified
full and empty capsids of AAV5, the most stable serotype, were tested
at starting concentrations of 5� 1013 viral genome (vg)/mL and 3.4�
1013 particles/mL, respectively. The samples serially diluted 10–100x
into PBS and followed by Tms determination identified a minimal
concentration at which signal could be measured. The lowest
detectable concentrations for the full and empty capsids were
5 � 1011 vg/mL and 3.4 � 1011 particles/mL, respectively, tested in
25 mL (Figures 4A and 4B).

AAV VP3 Is the Determinant of Capsid Stability

Following the observation that the genome had only a minor effect on
the AAV stability, the role of VP1, VP2, and VP3 on capsid stability
was analyzed for AAV2, the serotype exhibiting the lowest capsid
stability (Figure 1B; Table 1). AAV2 virus-like particles (VLPs)
assembled from (1) VP1, VP2, and VP3 (AAV2-VP123); (2) VP1
and VP3 only (AAV2-VP13), (3) VP2 and VP3 only (AAV2-
VP23), and (4) VP3 only (AAV2-VP3) were generated by the site-
directed mutagenesis of the start codon of the respective VP to be
eliminated in the pFBDVPm11 plasmid.24 The VLPs were produced
and purified, as described in Materials and Methods, and diluted into
PBS for Tm analysis by DSF. SDS-PAGE (silver stained) and negative-
stain EM showed the correct VP content for each construct and intact
capsid assembly (Figure 5A). The Tms for the WT VLPs and VP
variant VLPs were superposable and their mean Tm was �67.5�C ±

0.5�C (Figure 5B). In this assay, AAV5 VLPs were included as a con-
trol sample and its Tm was measured at 90�C ± 0.5�C, which is within
experimental error of the value obtained from the samples produced
in the OneBac system19 and used for the assays reported above (Fig-
ure 5B). These data showed that VP3 is sufficient to assemble the virus
capsid, as previously reported,25–27 and that its sequence is the sole
determinant of the capsid stability.
ber 2017



Figure 1. Sample Evaluation and Stability of Full rAAV1–rAAV9-gfp and rAAVrh.10-gfp, Packaging the GFP Transgene, Vectors in PBS

(A) Coomassie blue stained SDS-PAGE (left) and negative-stained EM (right) of rAAV1–rAAV9 and rAAVrh.10 as indicated above each panel. Scale bar, 100 nm, is shown in

theAAVrh.10EM image. (B) Thermal profile (shownasnormalized relative fluorescence units [RFUs]) versus temperature (T [�C]) of rAAV1–rAAV9and rAAVrh.10obtainedbyDSF
analysis. A representative profile is shown for each serotype. See also Table 1. Each profile is colored according to the serotype, as shown on the right-hand side.

www.moleculartherapy.org
The observation that VP3 was the determinant of AAV capsid stabil-
ity initiated a comparative analysis of the sequences of the AAVs.
The sequence identity between the ten AAVs was calculated using
the Clustal Omega application28 (data not shown), and calculation
of the isoelectric point (pI) and analysis of the number of basic and
acidic residues were conducted using the ExPASy application.29

The sequence identity between the AAVs range from�55%, between
AAV4 and AAV5 and between them and the other AAVs, to 99% be-
tween AAV1 and AAV6 (data not shown), consistent with previous
reports.1,18 A reversed relationship was observed between the Tm of
each AAV in PBS and UB when plotted with the calculated pI, with
the exceptions being AAV4 and AAV6 (Figure 6). These viruses
both had a higher pI than was expected in the overall trend, in which
Molecular Th
AAV5, with the lowest calculated pI, was the most stable serotype.
The data indicated a potential role of the acidic and basic residues
(reflected in the pI) in dictating the stability of the AAV capsid.

Tm Distinguishes a Single Acidic or Basic Amino Acid Residue

Difference in an AAV Variant

The validity of the prediction that VP3 sequence and pI, particularly
the ratio of basic to acidic resides, is a determinant of AAV stability,
was tested by comparing AAV1 and AAV6, which differ by six
amino acids, including one acidic/basic amino acid, E531K. Recip-
rocal variants, AAV1-E531K and AAV6-K531E30 and AAV1 and
AAV6 packing the luciferase gene were analyzed by DSF. The Tms
for AAV1, AAV1-K531, AAV6, and AAV6-E531 were 84.0�C,
erapy: Methods & Clinical Development Vol. 6 September 2017 173

http://www.moleculartherapy.org


Table 1. Tm of AAV1–AAV9 and AAVrh.10 Full and Empty Capsids in Different Buffers

Buffer AAV1 Full AAV1 Empty AAV2 Full AAV2 Empty AAV3 Full AAV3 Empty AAV4 Full AAV4 Empty AAV5 Full AAV5 Empty

PBS 83.5 ± 0.1 83.8 ± 0.3 68.2 ± 0.6 67.3 ± 0.8 71.7 ± 1.0 71.2 ± 1.2 75.0 ± 0.7 75.0 ± 0.5 89.2 ± 0.1 89.2 ± 0.3

CiPO4 83.0 ± 0.1 83.2 ± 0.6 67.2 ± 0.6 65.5 ± 0.9 67.8 ± 0.8 68.2 ± 0.3 73.3 ± 1.1 74.0 ± 0.5 89.2 ± 0.1 89.2 ± 0.3

HEPES 85.0 ± 0.1 85.0 ± 0.9 76.8 ± 0.3 77.5 ± 0.5 82.7 ± 0.6 83.0 ± 0.1 77.0 ± 0.7 76.0 ± 0.5 88.7 ± 0.1 88.7 ± 0.3

Tris 86.0 ± 0.1 85.0 ± 2.2 79.7 ± 0.3 80.2 ± 0.3 86.8 ± 0.3 86.8 ± 0.1 76.5 ± 2.1 77.5 ± 0.5 88.7 ± 0.3 88.7 ± 0.3

LR 84.5 ± 0.9 84.7 ± 0.6 75.2 ± 0.3 76.0 ± 1.8 78.5 ± 4.0 79.0 ± 2.5 75.3 ± 0.4 75.5 ± 0.5 89.0 ± 0.1 89.0 ± 0.1

BSS 84.3 ± 0.3 84.2 ± 0.3 71.2 ± 0.6 70.7 ± 1.8 76.3 ± 1.2 76.8 ± 0.3 75.5 ± 0.7 76.0 ± 0.5 89.3 ± 0.1 89.3 ± 0.3

UB 85.3 ± 0.3 85.0 ± 0.5 76.3 ± 0.3 75.0 ± 1.3 81.0 ± 0.9 82.5 ± 2.8 77.8 ± 0.4 77.5 ± 0.5 89.0 ± 0.1 89.0 ± 0.1

Buffer AAV6 Full AAV6 Empty AAV7 Full AAV7 Empty AAV8 Full AAV8 Empty AAV9 Full AAV9 Empty AAV10 Full AAV10 Empty

PBS 77.5 ± 0.6 78.5 ± 0.9 76.5 ± 0.1 76.7 ± 0.3 72.0 ± 0.1 71.2 ± 0.6 77.0 ± 0.3 77.0 ± 0.5 77.0 ± 0.8 77.0 ± 0.1

CiPO4 78.8 ± 1.3 79.3 ± 0.3 75.2 ± 0.3 75.0 ± 0.1 71.0 ± 0.3 71.2 ± 0.6 76.7 ± 0.3 76.5 ± 0.1 76.5 ± 0.1 76.0 ± 0.1

HEPES 81.3 ± 0.9 81.3 ± 0.5 76.5 ± 0.1 76.0 ± 0.1 72.0 ± 0.3 71.2 ± 0.6 77.3 ± 1.0 77.5 ± 0.3 77.5 ± 0.3 77.3 ± 0.3

Tris 80.7 ± 0.6 81.8 ± 1.2 78.0 ± 0.1 78.5 ± 0.1 73.5 ± 0.3 72.0 ± 0.9 78.2 ± 0.5 78.2 ± 0.3 78.2 ± 0.3 79.7 ± 0.6

LR 79.7 ± 2.2 80.2 ± 1.5 78.0 ± 0.1 78.0 ± 0.1 73.9 ± 1.0 72.7 ± 1.2 77.5 ± 0.3 78.3 ± 0.5 78.3 ± 0.5 78.3 ± 0.6

BSS 79.5 ± 0.5 79.5 ± 0.3 78.0 ± 0.1 77.3 ± 0.3 73.1 ± 0.3 72.5 ± 0.9 77.2 ± 0.5 78.0 ± 0.3 78.0 ± 0.3 78.8 ± 1.4

UB 80.8 ± 1.5 80.8 ± 3.0 78.5 ± 0.1 77.2 ± 0.3 73.3 ± 0.8 73.0 ± 0.1 77.5 ± 0.3 78.5 ± 0.9 78.5 ± 0.9 78.5 ± 0.6

Buffer abbreviations and formulations are provided in the Materials and Methods.

Molecular Therapy: Methods & Clinical Development
78.0�C, 79.0�C, and 83.5�C, respectively. The Tm for AAV1-K531 was
similar to that of AAV6, whereas that of AAV6-E531 was similar to
that of AAV1 (Figure 5C). Thus, mutation of AAV1 residue E531
to K resulted in destabilization, whereas mutation of AAV6 K531
to E resulted in stabilization (Figure 5C).

Capsid Stability in Different Buffer Formulations Shows No

Significant Effect on AAV Transduction Efficiency

To determine if the difference in stability observed in different buffer
formulations translated to transduction efficiency, luciferase gene
expression by four AAV serotypes belonging to group I (AAV2), II
(AAV1 and AAV8), and III (AAV5), diluted into the different buffers,
was tested in HEK293 cells. These four serotypes were selected not
only to represent the stability groups defined for the AAVs, but
also because they represent the range of sequence identity and struc-
tural diversity between the AAV serotypes. AAV2 transduces
HEK293 more efficiently than AAV1 (23% of AAV2), AAV5 (2%
of AAV2), and AAV8 (2% of AAV2) based on mean relative light
unit (RLU). Comparison of the transduction efficiency (TE) of all
four vectors, normalized to the PBS data, did not differ significantly
for each serotype in the respective buffers (Figure 7). Similarly, there
was no correlation between the Tm and TE of each AAV in the
different buffers, except for AAV8, which displayed a minor upward
trend (Figure 7). This observation is consistent with the cell culture
media, into which the viruses, previously exposed to different buffers,
are diluted by 10X, serving as the determinant of the virus properties
and not the formulation buffers. This observation was anticipated
because dilution of the viruses from Tris-HCl, utilized for neutraliza-
tion after purification, into the different formulation buffers dictated
their thermostability, as presented above. Thus, when working at a
physiological or close to physiological pH, AAV vector storage buffer
174 Molecular Therapy: Methods & Clinical Development Vol. 6 Septem
formulations dictate stability. However, the extracellular environ-
ment would dictate rAAV vector performance in vitro and likely
in vivo.

DISCUSSION
The use of AAVs as a clinical gene therapy vector requires good
manufacturing practice (GMP), with the characterization of the
final product to include certification of purity, stability, genome titer,
infectious titer, and absence of endotoxins, according to Food and
Drug Administration (FDA) requirements (reviewed by Wright31).
In this study, we developed a DSF protocol that determines the ther-
mal profile or Tm of AAV capsids as a method for serotype identifi-
cation. The reported dosage of AAVs utilized in several clinical and
preclinical trials is 1012–1013 vg/kg or 1011–1014 vg/patient.32–34

The application of DSF for serotype identification required minimal
samples of �1011 vg/mL or particles/mL for full and empty capsids,
respectively, in 22.5 mL of total volume to obtain a measurable fluo-
rescence enabling Tm calculation (Figures 4A and 4B). This amount
of material is easily attainable in therapeutic samples, making DSF
a suitable approach for the proposed serotype identification.

Significantly, the distinct Tm of each AAV serotype in different buffer
formulations enables their identification in�1 hr. The Tm of AAV1–
AAV9 and AAVrh.10 was a unique identifier for each serotype, with
the exception of AAV7, AAV9, and AAVrh.10 in PBS, which were
similar (Figure 1B; Table 1). These serotypes could, however, be
distinguished based on their Tm measured in other buffers (Figure 2;
Table 1). For example, AAV9 showed almost no variation in Tm in a
different buffer formulation, whereas AAV7 showed a 3�C variation
of Tm in the same buffers (Figures 2G and 2I), providing additional
means for distinguishing the two viruses. A previous comparative
ber 2017



Figure 2. Comparative Thermal Profiles of Full AAV1–AAV9-gfp and AAVrh.10-gfp Capsids in Commonly Used AAV Formulation and Storage Buffers and UB

(A–J) Comparison of (A) AAV1, (B) AAV2, (C) AAV3, (D) AAV4, (E) AAV5, (F) AAV6, (G) AAV7, (H) AAV8, (I) AAV9, and (J) AAVrh.10 thermal profiles (shown as in Figure 1) in

different buffers. Each buffer profile is colored according to the series legend in (K). (K) Discrete dots representing the distribution of Tms (
�C) for each AAV serotype in the

different buffers, as indicated to the right-hand side.

www.moleculartherapy.org
analysis of AAV capsid stability and capsid dynamics for AAV1,
AAV2, AAV5, and AAV8 introduced DSF as a method for distin-
guishing AAV serotypes based on stability.35 The Tm obtained for
AAV1, AAV2, AAV5, and AAV8 in this previous study35 in the
Molecular Th
PBS buffer used is consistent with our observations. In other studies
of AAV2 and AAV5 in the lactate ringer (LR) and balanced salt solu-
tion (BSS) buffers, similar Tms to those obtained in our study were re-
ported.36,37 More recently, another group utilized this DSF approach
erapy: Methods & Clinical Development Vol. 6 September 2017 175

http://www.moleculartherapy.org


Figure 3. Comparative Analysis of the Tm of Full, Packaging GFP Transgene, and Empty Capsids in the Different AAV Formulation and Storage Buffers

Plots show Tm (�C) (y axis) versus buffer (x axis) for two selected rAAV serotypes from the buffer stability groupings. Group I was AAVswith Tms varying by�15�C–20�C, AAV2
and AAV3 (top); group II was AAVs with Tms varying by�3�C–6�C, AAV8 and AAVrh.10 (middle); and group III was AAVswith Tms varying by <2.0

�C, AAV5 and AAV9. The Tm

of the full rAAV capsids is shown in a black line, and the empty capsids are shown in a gray line.

Molecular Therapy: Methods & Clinical Development
to identify AAV1, AAV2, AAV5, AAV6-K531E, AAV8, and AAV9.38

Significantly, these previous studies used different biological “repli-
cates” that were produced and purified using different protocols.
The similarity of Tms in the different buffers supports the validity
of the DSF approach for serotype identification.

In addition to there being no significant difference between full and
empty capsids (Figure 3; Table 1), the Tms for full capsids packaging
GFP or luciferase, e.g., AAV1 and AAV6, were the same in PBS (Fig-
176 Molecular Therapy: Methods & Clinical Development Vol. 6 Septem
ures 2A, 2F, and 5C). These data support the conclusion that the
encapsulated genome is not a determinant of AAV capsid thermosta-
bility. It was recently reported, based on atomic force microscopy
analysis of AAV2 empty capsids and those packaging single-stranded
DNA (ssDNA) or self complementary DNA (scDNA) genomes, that
the scDNA-containing capsid had greater resistance to deep deforma-
tion.39 This information was revealed by quantitative statistical
analysis because the observable correlations with genome content
were minimal.39 This observation implies that only a packaged
ber 2017



Figure 4. Concentration Survey of AAV5

(A) Full rAAV5-luc capsids at 5.0 � 1010–5.0 � 1012 vg/mL. (B) Empty rAAV5

capsids at 3.4 � 1011–3.4 � 1013 particles/mL. The inverted measured rate of

change of fluorescence with time, dRFU/dT, is shown plotted in the y axis against T

(�C) on the x axis.

www.moleculartherapy.org
double-stranded genome imparted mechanical AAV capsid stability,
not ssDNA, compared to empty capsids, as reported here.

The observation that VP3 content alone is the determinant of
AAV capsid stability ensures that vectors generated, with modified
quantities of VP1 and VP2, can be analyzed by DSF (Figures 5A and
5B). TheVP3 observation is consistent with previous reports, in which
AAV5 containing a reduced VP1 content mixed with AAV2 with a
higher VP1 content analyzed by DSF resulted in two distinct Tms, cor-
responding to the Tm of AAV2 and AAV5 when tested alone.35 These
observations expand the utility of DSF for identification of WT AAV
serotypes and chimeric or hybrid AAV vectors, which retain the com-
plete VP3 sequence of one serotype. This is important because vectors
with reduced VP1 content, often produced using the baculovirus/sf9,
as for example, AAV5 and AAV8,19,40,41 can be authenticated using
DSF. This method is also thus applicable for vectors containing the
VP1 of another serotype, e.g., the AAV2 VP1 incorporated into
AAV5 and AAV8, to improve their infectivity.41
Molecular Th
Previous analysis of the association energy and buried surface area for
the symmetry-related VP:VP interactions of AAV1, AAV2, AAV5,
and AAV8 capsids, based on the crystal structures, did not show
any correlation with AAV capsid stability.35,42 Data reported here
indicate that AAV serotype stability is based on the amino acid
sequence of VP3 and is governed by the ratio of basic:acidic residues,
which is correlated to the pI of the capsids (Figure 6). The reversibility
of the AAV1 and AAV6 Tms by the single E531K difference (Fig-
ure 5C) confirmed this observation. The Tm for the AAV6-E531
variant is higher than that of AAV6 and equivalent to that of
AAV1, whereas the Tm for the AAV1-K531 variant is equivalent to
that of AAV6 within the ± 0.5�C error associated with these measure-
ments. Thus, DSF has the ability to differentiate among AAVs that
differ by a single amino acid, provided the amino acid difference
causes a change in the overall charge and pI of the virus capsid.

The group I AAV serotypes, with highly variable Tms in the different
buffers, can have a broad tropism (e.g., AAV2)1 or limited host
tropism, for example, AAV3B.43 The group II AAV serotypes, with
intermediate variability in stability, can have limited tissue tropism,
e.g., AAV1 for skeletal muscle44 and AAV8, which targets the liver.45

Finally, group III AAV serotypes, displaying little to no change in Tm

in the different buffers, could also have broad (e.g., AAV9)46,47 or
limited tissue tropism (e.g., AAV5).1 These observations show that
storage buffer is not a determinant of tissue or cellular tropism, as
was observed in the lack of any significant correlation with the level
of gene expression in HEK293 cells (Figure 7). This suggests that
the cellular or tissue environment encountered during infection dic-
tates each AAV’s transduction efficiency, consistent with observed
differences in cell or tissue tropism during comparative infection
analysis.1,48

In summary, DSF offers a rapid, cost effective, and robust method for
AAV serotype identification in specific buffers because of their unique
thermal stability profiles in the commonly utilized formulation and
storage buffers. Table 1 reported here can serve as a “look up“ refer-
ence table for the AAV serotypes tested because the data presented are
reproducible, regardless of the source of sample production and
method utilized for purification. The observation that capsid stability
is based primarily on the charged VP3 residues ensures that Tm trends
can be predicted for novel capsid variants compared to the WT virus.
These data presented lead us to propose DSF as a method to be uti-
lized for AAV vector identification post-storage and pre-administra-
tion as part of the quality control protocol for preclinical and clinical
samples. Investigators should be able to add to the look up table for
additional AAV serotypes or novel vectors of interest to expand it
for all subsequent sample preparations.

MATERIALS AND METHODS
AAV Production

OneBac:Sf9 rep/cap producer cell lines of serotypes AAV1–AAV6,
AAV8, AAV9, and AAVrh.1019 were grown at 28�C in suspension
culture under constant agitation to 1 L at 1.0 � 106 cells/mL and
were infected with Bac-UF26-gfp at an MOI of 5.19,49 The infected
erapy: Methods & Clinical Development Vol. 6 September 2017 177

http://www.moleculartherapy.org


Figure 5. Sample Evaluation and Stability of WT and Mutant AAV2 VLPs

(A) Negative-stained EM (top) and silver-stained SDS-PAGE of AAV2-VP123 (WT),

AAV2-VP13, AAV2-VP23, and AAV2-VP3 VLPs (bottom). Top: white scale bar,

50 nm. Bottom: the position of VP1, VP2, and VP3 is indicated with arrows. (B)

Figure 6. AAV Capsid Tm Is pI Dependent

A comparative analysis of the Tm of rAAV1–rAAV9 and AAVrh.10 in PBS and UB is

plotted against the calculated capsid VP3 pI.

Molecular Therapy: Methods & Clinical Development

178 Molecular Therapy: Methods & Clinical Development Vol. 6 Septem
cells were harvested 72 hr post infection by centrifugation at 1.5K rpm
in a JA-20 rotor. A successful infection was characterized by a bright
green pellet due to intense GFP expression. The pellets were resus-
pended in TD buffer (1x PBS, 1 mM MgCl2, and 2.5 mM KCl), and
the supernatant was precipitated with 10% (w/v) PEG8000, as previ-
ously described.50 The cell pellets were subjected to three freeze-thaw
cycles in a dry ice/ethanol freezing bath and a 37�C water bath. After
the third freeze-thaw cycle, the cell pellet and resuspended polyeth-
ylene glycol (PEG) pellet were treated with Benzonase (250 U) and
incubated at 37�C for 30 min. Both solutions were clarified by centri-
fugation at 10,000 � g at 4�C for 20 min for purification (see below).

rAAV luciferase (rAAV1-luc, rAAV2-luc, rAAV5-luc, rAAV8-luc,
rAAV7-luc, rAAV6-luc, rAAV6-E531-luc, and rAAV1-K531-luc)
packaging vectors were produced by triple transfection in HEK293
cells. For this purpose, cells were seeded on 15-cm cell culture dishes.
At a confluency of �75%, the old growth medium was replaced with
15 mL of fresh DMEM. The three plasmids pHelper,51 pTR-UF3-luc,
and pXRAAV (for the respective virus as listed above) were mixed at
an equimolar ratio (total: 40 mg to be used per 15-cm plate) and
diluted in OptiMEM (Gibco) to a volume of 1 mL (per 15-cm plate).
After adding 125 mL of polyethyleneimine (1 mg/mL), the solution
was mixed, incubated at room temperature (RT) for 15 min, and
added dropwise to the HEK293 cells. The following day, 5 mL of fresh
DMEM were added to each plate. The cells were harvested after 72 hr
and treated as described above for the Sf9 cells.

The AAV2 VP variant VLPs were generated by site-directed muta-
genesis (Agilent) of the AAV2 plasmid pFBDVPm11.24 The VP1
Thermal profiles for AAV2-VP123 (WT), AAV2-VP13, AAV2-VP23, and AAV2-VP3

(different shades of blue), and rAAV5 (gray) VLPs. The AAV2 sample profiles are

superposable and have identical Tms of 67.5�C. (C) Thermal profiles (normalized

RFU v T [�C] of full capsids of rAAV1-luc [purple], rAAV1-K531-luc [purple broken],

rAAV6-luc [pink], and AAV1-E531-luc [pink broken]). The stabilizing/destabilizing

effect of E531K is evident.

ber 2017



Figure 7. Transduction Efficiency of rAAV Diluted into Different Buffers

The normalized relative fluorescence (RFU) in HEK293 cells is shown for rAAV1-luc, rAAV2-luc, rAAV5-luc, and rAAV8-luc post incubation in the different buffers (as indicated

on the right-hand side) above a plot of the Tm (left-hand side) and TE (right-hand side) against the same buffers. A similar trend in stability and TE is only observed for AAV8.

www.moleculartherapy.org
and VP2 start codons were mutated to GCG to generate AAV2-VP13,
AAV2-VP23, and AAV2-VP3 only constructs. The WT and mutant
plasmids were used to generate recombinant AAV2 VLPs in Sf9 cells
by the Bac-to-Bac expression system (Invitrogen) according to the
Molecular Th
manufacturer’s protocol. The infected Sf9 cells were harvested by
centrifugation at 1,100 � g for 20 min in a JA10 rotor. The pellets
were resuspended and prepared for purification as described above
for the samples produced in the Sf9 cell lines.
erapy: Methods & Clinical Development Vol. 6 September 2017 179

http://www.moleculartherapy.org


Molecular Therapy: Methods & Clinical Development
AAV Purification by AVB and Capture Select Affinity Ligand

Column Chromatography Followed by Sucrose Gradient

The clarified supernatants from the various virus production protocols
described abovewere diluted 1:1withTDbuffer and loaded onto a pre-
packed 1-mL AVB Sepharose HP column (GE Healthcare) (for
AAV1–AAV8 and AAVrh.10) or a gravity flow column packaged
from the capture select affinity ligand for AAV9 (CSAL9) at a
flow rate of 0.5 mL/min. After loading, the column was washed with
20 mL of TD buffer. The virus was eluted with elution buffer (0.1 M
NaAc and 0.75MNaCl, pH 2.5), and the peak fractions were collected
and neutralized with 1M Tris-HCl, pH 10 (neutralization buffer), at a
1:10 ratio. The elution fractions that showedVP1, VP2, andVP3 on an
SDS-PAGE gel were pooled, and the sample was concentrated to a vol-
ume of 500 mL and loaded onto a 5%–40% step sucrose gradient.
Empty and full virus capsids were separated by centrifugation at
35K rpm in an SW41 rotor for 3 hr at 4�C. The empty capsids were
extracted with a syringe from the 20%–25% sucrose fraction and the
full capsids from the 30% to 35% fraction. The samples were buffer
exchanged into 20 mM Tris-HCl, pH 7.4, and 150 mM NaCl and
concentrated by pelleting at 50K rpm in an SW51 rotor. The pellet
was resuspended in the Tris-HCl buffer, and the sample concentra-
tions were determined by UV spectrometry for the empty capsids
(E = 1.7 for concentration in mg/mL) and titers were determined by
qPCR for full capsids, as previously described.19

Determination of the Thermal Stability of AAV Capsids by DSF

This method monitors the binding of the SYPRO Orange dye to
hydrophobic regions of proteins that are exposed during unfolding.
For the comparative analysis of full and empty capsids, 2.5 mL
of each AAV serotype, at a concentration of 1 � 1014 vg/mL or
1 mg/mL (1 � 1014 particles), respectively, were added to 20 mL of
each of the six commonly used buffer formulations for AAV vector
storage and gene therapy applications and a newly developed buffer
called UB (see formulation below). This buffer was created to over-
come potential effects of temperature on pH when thermal stability
assays are conducted at low pH and was included here as a control.
The commonly used buffers include (1) PBS (10 mM Na2HPO4,
1.8 mMKH2PO4, pH 7.4, 27 mMKCl, and 137 mMNaCl), (2) citrate
phosphate (CiPO4) (0.2 M Na2HPO4 and 0.1 M citric acid, pH 7.4),
(3) HEPES (50 mM HEPES, pH 7.4, 150 mM NaCl, and 2 mM
MgCl2), (4) Tris-HCl (Tris) (20 mM Tris-HCl, pH 7.4, 150 mM
NaCl, and 2 mM MgCl), (5) Lactated Ringer (LR) (27.7 mM sodium
lactate, pH 6.5, 102.7 mM NaCl, 4.0 mM KCl, and 1 mM CaCl2), and
(6) balanced salt solution (BSS) (109.5 mM NaCl, 10.1 mM KCl,
3.3 mM CaCl2, 1.4 mM MgCl2, 28 mM sodium acetate, and
5.8 mM sodium citrate, pH 7.4, with 0.02% Tween). The formulation
for UB is 20 mM HEPES, 20 mM 2-(N-morpholino) ethanesulfonic
acid (MES), 20 mM sodium acetate, pH 7.4, 150 mM NaCl, and
5 mM CaCl2. In addition, 2.5 mL of 1% SYPRO Orange dye (Invitro-
gen) was added to each mixture to make a total reaction volume of
25 mL. The assays were run in a Bio-RadMyiQ2 Thermocycler instru-
ment, with temperature ranging from 30�C to 99�C and ramping at
0.5�C per step.35 This protocol can be adapted for any qPCR instru-
ment using filters commonly provided with the machines: FAM
180 Molecular Therapy: Methods & Clinical Development Vol. 6 Septem
(485 nm) for excitation and ROX (625 nm) for emission. The rate
of change of fluorescence with temperature was recorded, and the
thermal profile is output as�dRFU/dT versus temperature. The ther-
mal profile is then inverted by multiplying with �1 and normalized
by dividing the raw values of the profile by the peak dRFU/dT value
for evaluation. The peak value recorded on the thermogram is the Tm.
A negative control 22.5 mL of each buffer and 2.5 mL of SYPRO
Orange were included for each run. All experiments were conducted
in triplicate each time using at least two biological replicates for all the
samples tested, except for AAV4, which was repeated only twice with
one biological sample due to a low sample yield.

To survey the minimal concentration of AAV capsid that would
provide measurable fluorescence using DSF, AAV5, displaying the
highest Tm, was used. AAV5 full and empty capsids, purified from a
rAAV5-luc construct expressed in HEK293 cells, at 5 � 1013 vg/mL
and 3.4 � 1014 particles/mL, respectively, were serially diluted 10–
100x in PBS, and 22.5mLof eachdilutionwas used for theDSF analysis,
as described above. To determine the role of the AAV VPs in capsid
stability, WT AAV2 and VP variant VLPs were assayed, also in PBS,
at a concentration of 1 � 1013 particles/mL, as described above, but
without dilution because the samples were already in the assay buffer.
To determine the role of basic and acidic residues in capsid stability,
rAAV1-luc and rAAV6-luc and their variants, rAAV1-K531-luc and
rAAV6-E531, at concentrations of �1 � 1011–1 � 1012 vg/mL in
PBS, were assayed by DSF, also as described above.

Transduction of HEK293 Cells by rAAV-luc Vectors in Different

Buffer Formulations

The genome-containing titer of rAAV1-luc, rAAV2-luc, rAAV5-luc,
and rAAV8-luc vectors, with a packaged luciferase transgene, were
determined by qPCR, as previously described.19 For the transduction
assay, �2.5 � 104 HEK293 cells were seeded in a 96-well plate 1 day
prior to infection. On the day of infection, the rAAV vectors were
diluted into the six common AAV buffers plus UB (total volume:
10 mL) to infect cells at an MOI of 104 for AAV2 or 105 for AAV1,
AAV5, and AAV8. The difference in the MOI used for AAV2 and
the other AAVs stems from the higher transduction level observed
for AAV2 in vitro compared to the other AAV serotypes tested.1

The AAV-buffer mixtures were incubated at 4�C for 1 hr. Prior to
infection, 90 mL of DMEM supplemented with 2% FBS and 1% anti-
biotic and antimycotic (ABAM) was added to the mixtures. The old
media on the cells was discarded, and the virus-buffer-medium
mixture (total volume: 100 mL) was added to the cells. After incu-
bating the cells at 37�C and 5% CO2 for 48 hr, the medium was
removed and the cells were washed with PBS. For the luciferase assay,
the cells were lysed and the luminescence was determined using the
Luciferase Assay Kit (Promega), according to the manufacturer’s pro-
tocol, on a Synergy HTX plate reader (BioTek).

AUTHOR CONTRIBUTIONS
A.B. and M.M. contributed to study conception, Figures 1–7, and
manuscript preparation; S.P., A.J., and J.C.Y. contributed to Figures
1 and 2; B.L. and B.B. contributed to study conception; R.M. and
ber 2017



www.moleculartherapy.org
M.A.-M. are the grantees for this study and contributed to study
conception and manuscript preparation.

CONFLICTS OF INTEREST
M.A.-M. is an SAB member for AGTC, StrideBio, Inc., and Voyager
Therapeutics, Inc., is a consultant for Intima Biosciences, and has a
sponsored research agreement with AGTC, Adverum Biotechnol-
ogies, and Voyager Therapeutics, Inc. These companies have interest
in the development of AAV for gene delivery applications. M.A.-M.
and M.M. are inventors of AAV patents licensed to various biophar-
maceutical companies. M.A.-M. is a co-founder of StrideBio, Inc. This
is a biopharmaceutical company with interest in developing AAV
vectors for gene delivery application.

ACKNOWLEDGMENTS
We thank the University of Florida (UF) Interdisciplinary Center
for Biotechnology Research (ICBR) electron microscopy laboratory
for providing negative-stain EM services. We thank Joshua Hull for
technical services. This work was supported by NIH grants R01
GM109524 and R01 GM082946 to R.M. and M.A.-M.

REFERENCES
1. Gao, G., Vandenberghe, L.H., Alvira, M.R., Lu, Y., Calcedo, R., Zhou, X., andWilson,

J.M. (2004). Clades of adeno-associated viruses are widely disseminated in human
tissues. J. Virol. 78, 6381–6388.

2. Rose, J.A., Maizel, J.V., Jr., Inman, J.K., and Shatkin, A.J. (1971). Structural proteins of
adenovirus-associated viruses. J. Virol. 8, 766–770.

3. Snijder, J., van de Waterbeemd, M., Damoc, E., Denisov, E., Grinfeld, D., Bennett, A.,
Agbandje-McKenna, M., Makarov, A., and Heck, A.J. (2014). Defining the stoichiom-
etry and cargo load of viral and bacterial nanoparticles by Orbitrap mass spectrom-
etry. J. Am. Chem. Soc. 136, 7295–7299.

4. Girod, A., Wobus, C.E., Zádori, Z., Ried, M., Leike, K., Tijssen, P., Kleinschmidt, J.A.,
and Hallek, M. (2002). The VP1 capsid protein of adeno-associated virus type 2 is
carrying a phospholipase A2 domain required for virus infectivity. J. Gen. Virol.
83, 973–978.

5. Zádori, Z., Szelei, J., Lacoste, M.C., Li, Y., Gariépy, S., Raymond, P., Allaire, M., Nabi,
I.R., and Tijssen, P. (2001). A viral phospholipase A2 is required for parvovirus infec-
tivity. Dev. Cell 1, 291–302.

6. Hastie, E., and Samulski, R.J. (2015). Adeno-associated virus at 50: a golden anniver-
sary of discovery, research, and gene therapy success–a personal perspective. Hum.
Gene Ther. 26, 257–265.

7. Gray, J.T., and Zolotukhin, S. (2011). Design and construction of functional AAV
vectors. Methods Mol. Biol. 807, 25–46.

8. Flotte, T.R. (2005). Adeno-associated virus-based gene therapy for inherited disor-
ders. Pediatr. Res. 58, 1143–1147.

9. Srivastava, A. (2016). In vivo tissue-tropism of adeno-associated viral vectors. Curr.
Opin. Virol. 21, 75–80.

10. Chao, H., Liu, Y., Rabinowitz, J., Li, C., Samulski, R.J., andWalsh, C.E. (2000). Several
log increase in therapeutic transgene delivery by distinct adeno-associated viral sero-
type vectors. Mol. Ther. 2, 619–623.

11. Nathwani, A.C., Tuddenham, E.G., Rangarajan, S., Rosales, C., McIntosh, J., Linch,
D.C., Chowdary, P., Riddell, A., Pie, A.J., Harrington, C., et al. (2011). Adenovirus-
associated virus vector-mediated gene transfer in hemophilia B. N. Engl. J. Med.
365, 2357–2365.

12. Gaudet, D., Méthot, J., and Kastelein, J. (2012). Gene therapy for lipoprotein lipase
deficiency. Curr. Opin. Lipidol. 23, 310–320.

13. Tardieu, M., Zérah, M., Husson, B., de Bournonville, S., Deiva, K., Adamsbaum, C.,
Vincent, F., Hocquemiller, M., Broissand, C., Furlan, V., et al. (2014). Intracerebral
Molecular Th
administration of adeno-associated viral vector serotype rh.10 carrying human
SGSH and SUMF1 cDNAs in children with mucopolysaccharidosis type IIIA disease:
results of a phase I/II trial. Hum. Gene Ther. 25, 506–516.

14. Tseng, Y.S., Vliet, K.V., Rao, L., McKenna, R., Byrne, B.J., Asokan, A., and Agbandje-
McKenna, M. (2016). Generation and characterization of anti-adeno-associated virus
serotype 8 (AAV8) and anti-AAV9 monoclonal antibodies. J. Virol. Methods 236,
105–110.

15. Tseng, Y.S., and Agbandje-McKenna, M. (2014). Mapping the AAV capsid host anti-
body response toward the development of second generation gene delivery vectors.
Front. Immunol. 5, 9.

16. Wobus, C.E., Hügle-Dörr, B., Girod, A., Petersen, G., Hallek, M., and Kleinschmidt,
J.A. (2000). Monoclonal antibodies against the adeno-associated virus type 2
(AAV-2) capsid: epitope mapping and identification of capsid domains involved in
AAV-2-cell interaction and neutralization of AAV-2 infection. J. Virol. 74, 9281–
9293.

17. Kuck, D., Kern, A., and Kleinschmidt, J.A. (2007). Development of AAV serotype-
specific ELISAs using novel monoclonal antibodies. J. Virol. Methods 140, 17–24.

18. Van Vliet, K., Mohiuddin, Y., McClung, S., Blouin, V., Rolling, F., Moullier, P.,
Agbandje-McKenna, M., and Snyder, R.O. (2009). Adeno-associated virus capsid
serotype identification: analytical methods development and application. J. Virol.
Methods 159, 167–177.

19. Mietzsch, M., Grasse, S., Zurawski, C., Weger, S., Bennett, A., Agbandje-McKenna,
M., Muzyczka, N., Zolotukhin, S., and Heilbronn, R. (2014). OneBac: platform for
scalable and high-titer production of adeno-associated virus serotype 1-12 vectors
for gene therapy. Hum. Gene Ther. 25, 212–222.

20. Miller, E.B., Gurda-Whitaker, B., Govindasamy, L., McKenna, R., Zolotukhin, S.,
Muzyczka, N., and Agbandje-McKenna, M. (2006). Production, purification and pre-
liminary X-ray crystallographic studies of adeno-associated virus serotype 1. Acta
Crystallogr. Sect. F Struct. Biol. Cryst. Commun. 62, 1271–1274.

21. Huang, X., Hartley, A.V., Yin, Y., Herskowitz, J.H., Lah, J.J., and Ressler, K.J. (2013).
AAV2 production with optimized N/P ratio and PEI-mediated transfection results in
low toxicity and high titer for in vitro and in vivo applications. J. Virol. Methods 193,
270–277.

22. Rayaprolu, V., Kruse, S., Kant, R., Movahed, N., Brooke, D., and Bothner, B. (2014).
Fluorometric estimation of viral thermal stability. Biol. Protoc. 4, e1199.

23. Brooke, D., Mohaved, N., and Bothner, B. (2015). Universal buffers for use in
biochemistry and biophysical experiments. AIMS Biophysics 2, 336–342.

24. Urabe, M., Ding, C., and Kotin, R.M. (2002). Insect cells as a factory to produce
adeno-associated virus type 2 vectors. Hum. Gene Ther. 13, 1935–1943.

25. Warrington, K.H., Jr., Gorbatyuk, O.S., Harrison, J.K., Opie, S.R., Zolotukhin, S., and
Muzyczka, N. (2004). Adeno-associated virus type 2 VP2 capsid protein is nonessen-
tial and can tolerate large peptide insertions at its N terminus. J. Virol. 78, 6595–6609.

26. Rabinowitz, J.E., Xiao, W., and Samulski, R.J. (1999). Insertional mutagenesis of
AAV2 capsid and the production of recombinant virus. Virology 265, 274–285.

27. Sonntag, F., Schmidt, K., and Kleinschmidt, J.A. (2010). A viral assembly factor
promotes AAV2 capsid formation in the nucleolus. Proc. Natl. Acad. Sci. USA 107,
10220–10225.

28. Sievers, F., Wilm, A., Dineen, D., Gibson, T.J., Karplus, K., Li, W., Lopez, R.,
McWilliam, H., Remmert, M., Söding, J., et al. (2011). Fast, scalable generation of
high-quality protein multiple sequence alignments using Clustal Omega. Mol. Syst.
Biol. 7, 539.

29. Gasteiger, E., Gattiker, A., Hoogland, C., Ivanyi, I., Appel, R.D., and Bairoch, A.
(2003). ExPASy: the proteomics server for in-depth protein knowledge and analysis.
Nucleic Acids Res. 31, 3784–3788.

30. Wu, Z., Asokan, A., Grieger, J.C., Govindasamy, L., Agbandje-McKenna, M., and
Samulski, R.J. (2006). Single amino acid changes can influence titer, heparin binding,
and tissue tropism in different adeno-associated virus serotypes. J. Virol. 80, 11393–
11397.

31. Wright, J.F. (2008). Manufacturing and characterizing AAV-based vectors for use in
clinical studies. Gene Ther. 15, 840–848.

32. Aitken, M.L., Moss, R.B., Waltz, D.A., Dovey, M.E., Tonelli, M.R., McNamara, S.C.,
Gibson, R.L., Ramsey, B.W., Carter, B.J., and Reynolds, T.C. (2001). A phase I study
erapy: Methods & Clinical Development Vol. 6 September 2017 181

http://refhub.elsevier.com/S2329-0501(17)30086-4/sref1
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref1
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref1
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref2
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref2
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref3
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref3
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref3
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref3
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref4
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref4
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref4
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref4
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref5
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref5
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref5
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref6
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref6
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref6
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref7
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref7
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref8
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref8
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref9
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref9
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref10
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref10
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref10
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref11
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref11
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref11
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref11
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref12
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref12
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref13
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref13
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref13
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref13
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref13
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref14
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref14
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref14
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref14
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref15
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref15
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref15
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref16
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref16
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref16
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref16
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref16
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref17
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref17
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref18
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref18
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref18
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref18
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref19
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref19
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref19
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref19
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref20
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref20
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref20
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref20
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref21
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref21
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref21
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref21
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref22
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref22
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref23
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref23
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref24
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref24
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref25
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref25
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref25
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref26
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref26
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref27
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref27
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref27
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref28
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref28
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref28
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref28
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref29
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref29
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref29
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref30
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref30
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref30
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref30
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref31
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref31
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref32
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref32
http://www.moleculartherapy.org


Molecular Therapy: Methods & Clinical Development
of aerosolized administration of tgAAVCF to cystic fibrosis subjects with mild lung
disease. Hum. Gene Ther. 12, 1907–1916.

33. Flotte, T.R., and Mueller, C. (2011). Gene therapy for alpha-1 antitrypsin deficiency.
Hum. Mol. Genet. 20, R87–R92.

34. Bainbridge, J.W., Smith, A.J., Barker, S.S., Robbie, S., Henderson, R., Balaggan, K.,
Viswanathan, A., Holder, G.E., Stockman, A., Tyler, N., et al. (2008). Effect of gene
therapy on visual function in Leber’s congenital amaurosis. N. Engl. J. Med. 358,
2231–2239.

35. Rayaprolu, V., Kruse, S., Kant, R., Venkatakrishnan, B., Movahed, N., Brooke, D.,
Lins, B., Bennett, A., Potter, T., McKenna, R., et al. (2013). Comparative analysis of
adeno-associated virus capsid stability and dynamics. J. Virol. 87, 13150–13160.

36. Osting, S., Bennett, A., Power, S., Wackett, J., Hurley, S.A., Alexander, A.L.,
Agbandje-Mckena, M., and Burger, C. (2014). Differential effects of twoMRI contrast
agents on the integrity and distribution of rAAV2 and rAAV5 in the rat striatum.
Mol. Ther. Methods Clin. Dev. 1, 4.

37. Boye, S.L., Bennett, A., Scalabrino, M.L., McCullough, K.T., Van Vliet, K.,
Choudhury, S., Ruan, Q., Peterson, J., Agbandje-McKenna, M., and Boye, S.E.
(2016). Impact of heparan sulfate binding on transduction of retina by recombinant
adeno-associated virus vectors. J. Virol. 90, 4215–4231.

38. Pacouret, S., Bouzelha, M., Shelke, R., Andres-Mateos, E., Xiao, R., Maurer, A., Mevel,
M., Turunen, H., Barungi, T., Penaud-Budloo, M., et al. (2017). AAV-ID: a rapid and
robust assay for batch-to-batch consistency evaluation of AAV preparations. Mol.
Ther. 25, 1375–1386.

39. Zeng, C., Moller-Tank, S., Asokan, A., and Dragnea, B. (2017). Probing the link
among genomic cargo, contact mechanics, and nanoindentation in recombinant
adeno-associated virus 2. J. Phys. Chem. B 121, 1843–1853.

40. Mietzsch, M., Casteleyn, V., Weger, S., Zolotukhin, S., and Heilbronn, R. (2015).
OneBac 2.0: Sf9 cell lines for production of AAV5 vectors with enhanced infectivity
and minimal encapsidation of foreign DNA. Hum. Gene Ther. 26, 688–697.

41. Kohlbrenner, E., Aslanidi, G., Nash, K., Shklyaev, S., Campbell-Thompson, M.,
Byrne, B.J., Snyder, R.O., Muzyczka, N., Warrington, K.H., Jr., and Zolotukhin, S.
(2005). Successful production of pseudotyped rAAV vectors using a modified bacu-
lovirus expression system. Mol. Ther. 12, 1217–1225.
182 Molecular Therapy: Methods & Clinical Development Vol. 6 Septem
42. Govindasamy, L., Padron, E., McKenna, R., Muzyczka, N., Kaludov, N., Chiorini, J.A.,
and Agbandje-McKenna, M. (2006). Structurally mapping the diverse phenotype of
adeno-associated virus serotype 4. J. Virol. 80, 11556–11570.

43. Ling, C., Lu, Y., Cheng, B., McGoogan, K.E., Gee, S.W., Ma, W., Li, B., Aslanidi, G.V.,
and Srivastava, A. (2011). High-efficiency transduction of liver cancer cells by recom-
binant adeno-associated virus serotype 3 vectors. J. Vis. Exp. 2538.

44. Elmallah, M.K., Falk, D.J., Nayak, S., Federico, R.A., Sandhu, M.S., Poirier, A., Byrne,
B.J., and Fuller, D.D. (2014). Sustained correction of motoneuron histopathology
following intramuscular delivery of AAV in pompe mice. Mol. Ther. 22, 702–712.

45. Graham, T., McIntosh, J., Work, L.M., Nathwani, A., and Baker, A.H. (2008).
Performance of AAV8 vectors expressing human factor IX from a hepatic-selective
promoter following intravenous injection into rats. Genet. Vaccines Ther. 6, 9.

46. Chen, B.D., He, C.H., Chen, X.C., Pan, S., Liu, F., Ma, X., Li, X.M., Gai, M.T., Tao, J.,
Ma, Y.T., et al. (2015). Targeting transgene to the heart and liver with AAV9 by
different promoters. Clin. Exp. Pharmacol. Physiol. 42, 1108–1117.

47. Dashkoff, J., Lerner, E.P., Truong, N., Klickstein, J.A., Fan, Z., Mu, D., Maguire, C.A.,
Hyman, B.T., and Hudry, E. (2016). Tailored transgene expression to specific cell
types in the central nervous system after peripheral injection with AAV9. Mol.
Ther. Methods Clin. Dev. 3, 16081.

48. Zincarelli, C., Soltys, S., Rengo, G., and Rabinowitz, J.E. (2008). Analysis of AAV se-
rotypes 1-9 mediated gene expression and tropism in mice after systemic injection.
Mol. Ther. 16, 1073–1080.

49. Aslanidi, G., Lamb, K., and Zolotukhin, S. (2009). An inducible system for highly effi-
cient production of recombinant adeno-associated virus (rAAV) vectors in insect Sf9
cells. Proc. Natl. Acad. Sci. USA 106, 5059–5064.

50. Zolotukhin, S., Potter, M., Zolotukhin, I., Sakai, Y., Loiler, S., Fraites, T.J., Jr., Chiodo,
V.A., Phillipsberg, T., Muzyczka, N., Hauswirth, W.W., et al. (2002). Production and
purification of serotype 1, 2, and 5 recombinant adeno-associated viral vectors.
Methods 28, 158–167.

51. Xiao, X., Li, J., and Samulski, R.J. (1998). Production of high-titer recombinant
adeno-associated virus vectors in the absence of helper adenovirus. J. Virol. 72,
2224–2232.
ber 2017

http://refhub.elsevier.com/S2329-0501(17)30086-4/sref32
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref32
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref33
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref33
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref34
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref34
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref34
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref34
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref35
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref35
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref35
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref36
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref36
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref36
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref36
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref37
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref37
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref37
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref37
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref38
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref38
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref38
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref38
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref39
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref39
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref39
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref40
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref40
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref40
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref41
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref41
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref41
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref41
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref42
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref42
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref42
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref43
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref43
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref43
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref44
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref44
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref44
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref45
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref45
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref45
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref46
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref46
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref46
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref47
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref47
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref47
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref47
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref48
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref48
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref48
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref49
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref49
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref49
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref50
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref50
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref50
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref50
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref51
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref51
http://refhub.elsevier.com/S2329-0501(17)30086-4/sref51

	Thermal Stability as a Determinant of AAV Serotype Identity
	Introduction
	Results
	Stability of rAAV1–rAAV9 and rAAVrh.10 in PBS Buffer Shows Disparate Profiles
	Comparative Stability Analysis of rAAV1–rAAV9 and rAAVrh.10 in Commonly Used Formulation and Storage Buffers Reveals Seroty ...
	Small Volume and Low Concentration Requirement of AAV Samples for DSF Analysis
	AAV VP3 Is the Determinant of Capsid Stability
	Tm Distinguishes a Single Acidic or Basic Amino Acid Residue Difference in an AAV Variant
	Capsid Stability in Different Buffer Formulations Shows No Significant Effect on AAV Transduction Efficiency

	Discussion
	Materials and Methods
	AAV Production
	AAV Purification by AVB and Capture Select Affinity Ligand Column Chromatography Followed by Sucrose Gradient
	Determination of the Thermal Stability of AAV Capsids by DSF
	Transduction of HEK293 Cells by rAAV-luc Vectors in Different Buffer Formulations

	Author Contributions
	Conflicts of Interest
	Acknowledgments
	References