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Antimicrobial Agents and Chemotherapy, July 2000, p. 1954-1960, Vol. 44, No. 7
0066-4804/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.
Sodium Dodecyl Sulfate and C31G as Microbicidal
Alternatives to Nonoxynol 9: Comparative Sensitivity of Primary Human
Vaginal Keratinocytes
Fred C.
Krebs,1
Shendra R.
Miller,1
Bradley J.
Catalone,1
Patricia A.
Welsh,1
Daniel
Malamud,2,3
Mary K.
Howett,1 and
Brian
Wigdahl1,*
Department of Microbiology and Immunology,
College of Medicine, The Pennsylvania State University, Hershey,
Pennsylvania 17033,1 and Department of
Biochemistry, School of Dental Medicine, University of
Pennsylvania,2 and Biosyn,
Inc.,3 Philadelphia, Pennsylvania 19104
Received 16 November 1999/Returned for modification 19 January
2000/Accepted 25 April 2000
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ABSTRACT |
A broad-spectrum vaginal microbicide must be effective against a
variety of sexually transmitted disease pathogens and be minimally
toxic to the cell types found within the vaginal epithelium, including
vaginal keratinocytes. We assessed the sensitivity of primary human
vaginal keratinocytes to potential topical vaginal microbicides
nonoxynol-9 (N-9), C31G, and sodium dodecyl sulfate (SDS). Direct
immunofluorescence and fluorescence-activated cell sorting analyses
demonstrated that primary vaginal keratinocytes expressed epithelial
cell-specific keratin proteins. Experiments that compared vaginal
keratinocyte sensitivity to each agent during a continuous, 48-h
exposure demonstrated that primary vaginal keratinocytes were almost
five times more sensitive to N-9 than to either C31G or SDS. To
evaluate the effect of multiple microbicide exposures on cell
viability, primary vaginal keratinocytes were exposed to N-9, C31G, or
SDS three times during a 78-h period. In these experiments, cells were
considerably more sensitive to C31G than to N-9 or SDS at lower
concentrations within the range tested. When agent concentrations were
chosen to result in an endpoint of 25% viability after three daily
exposures, each exposure decreased cell viability at the same constant
rate. When time-dependent sensitivity during a continuous 48-h exposure
was examined, exposure to C31G for 18 h resulted in losses in cell
viability not caused by either N-9 or SDS until at least 24 to 48 h. Cumulatively, these results reveal important variations in time- and
concentration-dependent sensitivity to N-9, C31G, or SDS within
populations of primary human vaginal keratinocytes cultured in vitro.
These investigations represent initial steps toward both in vitro
modeling of the vaginal microenvironment and studies of factors that
impact the in vivo efficacy of vaginal topical microbicides.
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INTRODUCTION |
The global spread of the human
immunodeficiency virus type 1 (HIV-1) has recently been driven by a
dramatic increase in heterosexual transmission, which is the
predominant route of transmission in developing countries
(8). This disturbing trend in the AIDS epidemic has
highlighted the necessity for additional measures to control the
transmission of HIV-1, including the development and distribution of
broad-spectrum, topical vaginal microbicides for use during
heterosexual intercourse (7). An ideal microbicide would be
female-controlled, broadly effective against HIV-1 as well as other
sexually transmitted disease (STD) pathogens such as human
papillomavirus (HPV) and herpes simplex virus types 1 and 2 (HSV-1 and
HSV-2, respectively), inexpensive, easy to use and store, and safe
during repeated and long-term use.
Products containing nonoxynol-9 (N-9), a widely available, commercially
marketed spermicidal agent, have been tested for microbicidal use. N-9
has in vitro activity against several STD pathogens, including HIV-1
(3, 9), but cannot be classified as broadly effective, since
it has no activity against nonenveloped viruses such as HPV
(4). In vivo effectiveness of N-9 as a microbicide is
unclear. Clinical studies have provided conflicting indications of N-9
effectiveness against transmission of HIV-1 and other STD pathogens
(2, 10, 11, 15, 20, 27). Results from human and animal
studies also indicate a narrow margin between N-9 effectiveness and
safety (22), as well as associations between N-9 use and vaginal irritation, inflammation, tissue infiltration by host immune
cells, and changes in vaginal flora (10, 16, 21, 22, 24).
These adverse effects may increase the risk for HIV-1 transmission
during sexual intercourse.
Because of the limitations of N-9 as a microbicidal agent, efforts have
been directed toward the development of second-generation microbicidal
agents with broader activity and lower toxicity. Our efforts have
focused on characterizing the in vitro virucidal potential of and
inherent cellular sensitivity to C31G and sodium dodecyl sulfate (SDS),
novel microbicidal agents that demonstrate activity against a broad
spectrum of STD pathogens, including HIV-1. C31G (in our present
studies) is an equimolar mixture of two amphoteric, surface-active
molecules: a C14 alkyl amine oxide and a C16
alkyl betaine. C31G is a broad-spectrum antimicrobial and spermicidal
agent (1, 5, 9, 25). However, like N-9, C31G has no activity
against HPV (5), a sexually transmitted virus that has a
direct causative role in the development of human cervical cancer. SDS,
an alkyl sulfate commonly used in research applications and in
commercially available personal hygiene products, is significantly less
cytotoxic than either N-9 or C31G and is effective against HIV-1,
HSV-2, and, importantly, papillomaviruses from several species,
including humans (5, 9). Other investigators (18; J. Piret, A. Desormeaux, P. Gourde, and M. G. Bergeron, Abstr. 38th Intersci. Conf. Antimicrob. Agents Chemother.,
abstr. H-8, 1998) have subsequently confirmed our original observations regarding the activity of SDS against HIV-1 and HSV-2 infectivity (National Institute of Allergy and Infectious Diseases Preclinical Topical Microbicides Workshop, May 1998) (5, 9, 12).
The present studies were performed to compare the sensitivity of
primary human vaginal keratinocytes to N-9, C31G, or SDS exposure.
Primary vaginal epithelial cells provide a realistic target for studies
of microbicidal cytotoxicity, since, as progenitors of the stratified
epithelium that lines the vagina, these cells form part of the physical
barrier which impedes the infection of HIV-1-susceptible target cells
such as dendritic cells (23), tissue macrophages, and
CD4-positive lymphocytes (28). Compromise of this barrier by
trauma or cellular damage that may accompany microbicide use could
therefore increase the risk of HIV-1 infection. The results reported
herein demonstrate that primary vaginal keratinocytes were less
sensitive to SDS exposure than to either N-9 or C31G exposure. Time-
and concentration-dependent differences in the cytotoxicity of N-9,
C31G, and SDS were also observed.
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MATERIALS AND METHODS |
Tissue isolation and cell culture.
Primary human vaginal
keratinocytes were isolated from the vaginal wall of tissues removed
during reconstructive surgeries. The average donor age was 63 years
(range, 25 to 79 years). Tissue samples were stored (for up to 2 h) at 4°C in minimal essential medium supplemented with penicillin
and streptomycin (0.08 mg/ml each), gentamycin (0.4 mg/ml), fungizone
(2.5 µg/ml), sodium bicarbonate (0.05%), and HEPES (10 mM) prior to
use. Vaginal tissues were cut full-thickness and washed two times in
phosphate-buffered saline (PBS). Tissues were digested overnight at
4°C and then at 37°C for 15 to 20 min in 0.25% trypsin-0.01%
EDTA in Hanks' balanced salt solution (Clonetics). Following
digestion, tissues were transferred to tissue culture dishes containing
2 ml of fetal bovine serum (HyClone) and 2 ml of defined keratinocyte
growth medium (KGM; Clonetics). Keratinocytes were then scraped away from the dermis with blunt-tipped forceps, washed, pelleted, and plated
in KGM (without serum) at a density of 2,500 cells/cm2 in
T-25 tissue culture flasks (for fluorescence-activated cell sorting
[FACS] analysis), 35-mm culture dishes (for immunofluorescence), or
12-well tissue culture plates [for
3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide (MTT)
analyses]. The medium was changed 24 h after seeding and twice
weekly thereafter. Primary, subconfluent keratinocyte cultures were
maintained for 10 to 14 days prior to experimental use. To decrease the
contributions of variations between donors, each set of experiments was
performed using cell populations from 2 to 5 donors.
Flow cytometric analyses.
Primary vaginal keratinocyte cell
populations were analyzed using fluorescence-activated cell sorting
(FACS). A monoclonal, fluorescein isothiocyanate-conjugated, anti-human
pan cytokeratin antibody (mouse immunoglobulin G1 [IgG1] isotype;
Sigma) was used to identify cells expressing a broad spectrum of human
cytokeratins. This antibody reacts with simple, cornifying and
noncornifying squamous epithelia and pseudostratified epithelia but not
with nonepithelial human tissues. CD4 expression was assessed using an
fluorescein isothiocyanate-conjugated, anti-human CD4 monoclonal antibody (mouse IgG1 isotype; BD PharMingen). Fibronectin expression was quantitated using a monoclonal, mouse anti-human fibronectin antibody (IgG1 isotype; Sigma) and an FITC-conjugated anti-mouse secondary antibody (isotype IgG1; Boehringer Mannheim). Trypsinized cells were fixed in 2% paraformaldehyde for 30 min at 4°C and washed
twice with PBS. Following a 1-h incubation period at 4°C with each
antibody (diluted 1:7.5), the cells were washed twice with PBS prior to
suspension in 2% paraformaldehyde and FACS analysis. For fibronectin
detection, the secondary antibody was introduced in a second 1-h
incubation period prior to final fixation.
Cell-surface marker identification by immunofluorescence.
Primary vaginal keratinocytes were characterized with respect to
keratin and CD4 expression by direct fluorescence using the keratin-
and CD4-specific antibodies described above. Cells cultured in 35-mm
tissue culture dishes were fixed and stained as described above.
Determination of cellular sensitivity to microbicide
exposure.
The effect of each agent on keratinocyte viability was
determined by monitoring MTT cleavage by mitochondrial dehydrogenases in viable cells, yielding a measurable, purple product (formazan) (17). Formazan production is proportional to the viable cell number and inversely proportional to the degree of cytotoxicity. N-9
(FW 616), C31G (C14 amine oxide [FW 257] and
C16 betaine [FW 327]), and SDS (FW 288) were obtained
from Biosyn, Inc., as 1% stock solutions. To eliminate the potential
effects of cell confluence and keratinization on cellular sensitivity,
each experiment was initiated and concluded before keratinocytes
reached confluence. For each experiment, agents were filter sterilized,
diluted in sterile water, and added (10 µl per 2 ml of medium) to
triplicate wells of subconfluent keratinocytes in KGM at the indicated
concentrations. Cells were incubated in the absence or presence of each
agent at 37°C in 5% CO2 and 90% humidity. At the
conclusion of each experiment, 250 µl of MTT (5 mg/ml) was added to
each well and incubated for 3 h at 37°C. Following removal of
the medium, intracellular formazan crystals were solubilized for 5 min
in 1 ml of 10% Triton X-100 in acidified isopropanol (0.1 N). The
resulting solutions were assayed spectrophotometrically at 570 nm and
corrected for nonspecific absorption at 690 nm. Statistical analyses
were performed using Microsoft Excel.
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RESULTS |
Primary vaginal keratinocytes express keratin.
To verify the
identity of cell populations derived from the vaginal tissues, cells
used for the assessment of cellular sensitivity to candidate
microbicides were characterized for the expression of cellular markers
using FACS analysis. A broad-spectrum anti-cytokeratin antibody was
selected to verify the presence of keratinocytes. Keratins comprise a
heterogeneous family of proteins whose expression is limited almost
exclusively to epithelial cells. Since keratinocytes do not express
CD4, an antibody specific for CD4 was used both as a negative control
and to detect contaminating immune cell types (i.e., T lymphocytes and
cells of monocyte or macrophage lineage). An antibody directed against
fibronectin was used as a nonreactive, isotype-matched negative control.
FACS analyses of primary vaginal keratinocytes demonstrated that these
cells express members of the keratin protein family (Fig.
1). Approximately 85% of the total cell
population expressed keratins above background levels. Keratin
expression in primary vaginal keratinocytes was heterogeneous, with
levels of expression spanning over two logs of intensity. Similar
patterns of keratin expression were observed using the AE3 antibody
(ICN Biomedicals, Inc.), which is specific to basic forms of keratin
(data not shown). CD4 or fibronectin expression was not detected.
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FIG. 1.
Primary human vaginal keratinocytes express members of
the keratin protein family. Primary vaginal keratinocytes were examined
using flow cytometry for expression of CD4, members of the keratin
protein family, or fibronectin. Analyses were conducted as described in
Materials and Methods. The horizontal and vertical axes represent
fluorescence intensity (log scale) and cell counts, respectively.
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Primary human vaginal keratinocytes were also characterized using
visible light microscopy (Fig.
2A) and
direct immunofluorescence
(Fig.
2B to D). Like the FACS analyses,
direct immunofluorescence
of primary vaginal keratinocytes revealed
expression of the keratin
protein family. Keratin expression in vaginal
keratinocytes (Fig.
2D) was readily detectable. The apparent
cytoplasmic localization
was consistent with the role of keratins as
intracellular intermediate
filaments. The heterogeneous levels of
fluorescence observed in
the vaginal keratinocytes paralleled the
spectrum of keratin expression
observed in the FACS analyses. No
autofluorescence was observed
(Fig.
2B). No CD4 expression was
detectable on the majority of
the cells examined. However, a small
number of cells did appear
to be weakly positive for CD4 (Fig.
2C).
These cells were distinct
in size and shape from the vast majority of
cells observed under
both visible light (Fig.
2A) and by direct
immunofluorescence
(Fig.
2D), suggesting that they may have been cells
of a different
type. Unlike the field illustrated in Fig.
2C, most of
the observable
fields were devoid of cells positive for CD4 expression,
indicating
that the number of CD4-positive cells was low (as also
suggested
by the FACS analyses). Because of their low number, these
cells
were not characterized further with respect to these studies.
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FIG. 2.
Keratin expression in primary human vaginal
keratinocytes can be identified by immunofluorescence. Primary vaginal
keratinocytes were examined by direct immunofluorescence for expression
of CD4 and members of the keratin protein family. Analyses were
conducted as described in Materials and Methods. (A) Representative
field under visible light; (B, C, and D) direct immunofluorescent
micrographs of vaginal keratinocytes in the absence of antibody,
labeled with CD4 antibodies, or labeled with pan cytokeratin
antibodies, respectively. The arrow in panel C indicates a cell weakly
positive for CD4 expression. The field of cells in panel C was selected
specifically to show the cells that expressed low levels of CD4 and is
not representative of a typical field; cells in most fields were devoid
of any detectable CD4 expression.
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Primary cultures of human vaginal keratinocytes are much less
sensitive to SDS or C31G than to N-9.
To determine the sensitivity
of vaginal keratinocytes to N-9, C31G, or SDS, primary cultures of
human vaginal keratinocytes were incubated with each agent and cell
viability was evaluated after 48 h of continuous exposure (Fig.
3). Over the concentration range examined
(2.5 × 10
4% to 5 × 103%),
C31G and SDS were equally cytotoxic (Fig. 3A). Exposure to either C31G
or SDS at 2.5 × 104% resulted in no decreases in
cell viability. However, at 1.25 × 103%, the
presence of either C31G or SDS reduced the number of viable cells to
approximately 7 or 3% of the number of control cells, respectively. At
the highest concentrations of C31G or SDS (2.5 × 103% or 5 × 103%), viable cells
were not detected after 48 h of exposure.
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FIG. 3.
Primary keratinocytes are more sensitive to N-9 than to
C31G or SDS during long-term exposure. Primary human vaginal
keratinocytes were exposed to N-9, C31G, or SDS for 48 h and
subsequently assessed for viability using MTT assays. (A) Cell survival
following exposure to concentrations of 2.5 × 104
to 5 × 103%; (B) Cell survival following exposure
to N-9 at concentrations of 2.5 × 105 to 2.5 × 104%. The arrows in panels A and B both indicate cell
viability at 2.5 × 104%. Cell viability following
microbicide exposure is expressed as the fraction of viable cells
relative to the number of mock-exposed cells. The results illustrated
are averages from two experiments in which triplicate wells for each
concentration were assayed.
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Primary human vaginal keratinocytes were particularly sensitive to the
presence of N-9. At a concentration of 2.5 × 10
4%,
N-9 reduced cell viability to 11% (Fig.
3A). In sharp contrast,
exposure to either C31G or SDS at the same concentration resulted
in
negligible cytotoxicity. To further explore the cytotoxicity
of N-9,
additional MTT experiments using lower concentrations
of N-9 were
performed (Fig.
3B). In these analyses, a 50% reduction
in
concentration, from 2.5 × 10
4% to 1.25 × 10
4%, resulted in an eightfold increase in cell
viability (to 64%).
Even at the lowest concentration tested (2.5 × 10
5%), cell viability was only 85%. Comparing
concentrations which
would be expected to result in a 50% reduction in
cell viability
(50% cytotoxicity concentration [TC
50]),
vaginal keratinocytes
were almost five times more sensitive to N-9
(TC
50 = 1.6 × 10
4%) than to
either C31G (TC
50 = 7.4 × 10
4%)
or SDS (TC
50 = 7.8 × 10
4%) during
long-term (48 h)
exposure.
Repetitive exposure to N-9, C31G, or SDS affects the viability of
primary keratinocytes.
Repeated application of microbicidal
products may result in toxic effects not evident after single or
infrequent use. Indeed, increased epithelial disruption was evident in
women who used N-9 daily for 2 weeks (19). In addition, a
recent animal study demonstrated that repeated application of N-9 was
detrimental to vaginal epithelial tissues (16). To evaluate
the in vitro cytotoxicity of N-9, C31G, or SDS after repeated exposure,
primary vaginal keratinocytes were exposed to three daily applications of each agent (Fig. 4). Each application
cycle consisted of a 2-h exposure followed by a wash with PBS and a
24-h incubation in new media. Following the third cycle, cell viability
was assessed by MTT assay. Results of these experiments indicated that
between 2.5 × 104 and 1.25 × 103%, repeated exposure to either N-9 or SDS resulted in
minimal reductions in cell viability. However, above 1.25 × 103%, viability in the presence of N-9 decreased sharply
to undetectable levels. A similar decrease in viability was observed in
the presence of SDS, but the sharp decline occurred at twice the
concentration. Cells were less sensitive to N-9 and SDS than to C31G
under these in vitro conditions. Although cell mortality following
repeated exposure to the lowest concentration of C31G was minimal,
viability decreased dramatically at higher concentrations and was
undetectable at and above 1.25 × 103%.
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FIG. 4.
Repetitive microbicide exposure affects the viability of
human vaginal keratinocytes. Primary human vaginal keratinocytes were
exposed to N-9, C31G, or SDS for 2 h. The cells were then washed
once with PBS and cultured under new medium for 24 h. This cycle
of exposure and recovery was repeated two more times. Cell survival was
assessed using MTT assays following the third exposure/recovery cycle.
Cell viability following microbicide exposure is expressed as the
fraction of viable cells relative to the number of mock-exposed cells.
The results illustrated are averages from two experiments in which
triplicate wells for each concentration were assayed.
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Repetitive in vitro exposure to N-9, C31G, or SDS results in
steadily increasing cytotoxicity.
Although the preceding
experiment demonstrated concentration-dependent cytotoxicity as a
consequence of repeated microbicide exposure, it did not address the
contribution of each application to the cumulative loss of cell
viability. To examine the contribution of each exposure cycle to the
total cytotoxicity, primary vaginal keratinocytes were subjected to the
same multiple application protocol as in the preceding experiment and
assessed for viability following the 24-h recovery period in each
application cycle. The results illustrated in Fig. 4 were used to
select concentrations at which multiple exposures to each microbicide
resulted in 25% cell viability (TC75). These
concentrations were selected to provide a low yet measurable level of
cell viability at the endpoints of each experiment as well as
detectable losses in cell viability at early time points. The
calculated TC75 of N-9 and SDS after the three 2-h
microbicide exposures were approximately 3.7- and 7.3-fold higher than
the TC75 of C31G, reflecting the higher cytotoxicity of
C31G under these conditions. Results indicated that each exposure cycle
during the 3-day exposure protocol contributed equally toward the total
amount of cytotoxicity (Fig. 5). Daily
incubation with N-9, C31G, or SDS resulted in a linear decrease in cell
viability.
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FIG. 5.
Repetitive microbicide exposure results in a steady
reduction in human vaginal keratinocyte viability. TC75
were determined from the results illustrated in Fig. 4. Cell survival
was assessed by MTT assay after each exposure and recovery cycle. The
cell viability following microbicide exposure is expressed as the
fraction of viable cells relative to the number of mock-exposed cells.
The results illustrated are averages from two experiments in which
triplicate wells for each concentration were assayed.
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Decreased cell viability during continuous exposure to C31G occurs
earlier than similar decreases after N-9 or SDS exposure.
Cytotoxicity during continuous exposure must also be considered in the
evaluation of chemical agents as potential microbicides, since
significant levels of microbicides are likely retained in the vagina
hours after the initial application (14). To determine the
time course of microbicide cytotoxicity during continuous exposure,
primary vaginal keratinocytes were exposed to a single concentration of
N-9, C31G, or SDS and assessed for cell viability 2, 8, 16, 24, and
48 h after the application of each microbicide. The results
depicted in Fig. 3A and B were used to select concentrations at which
exposure to each microbicide reduced cell viability to 25%
(TC75). The TC75 of C31G and SDS were
approximately fivefold higher than the TC75 of N-9,
reflecting the cytotoxicity of N-9 at low concentrations. Despite the
fivefold difference in concentration, N-9 or SDS exposure resulted in
similar levels of time-dependent cytotoxicity (Fig.
6). During the first 24 h of
exposure to either N-9 or SDS, cell viability was generally constant
and did not decrease below 76%. Between 24 and 48 h, cell
viability decreased at a much higher rate. By 48 h, the presence
of N-9 or SDS reduced cell viability to 5 and 11%, respectively. In
contrast, cell viability in the presence of C31G decreased linearly
after a 2-h exposure and was reduced to 4% by 16 h. These results
indicate that in vitro exposure to C31G leads to a more rapid decline
in cell viability than exposure to SDS, despite similar levels of
cellular sensitivity following long-term (48 h) exposure.
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FIG. 6.
Microbicide toxicity increases with continued exposure
to equivalent concentrations of N-9, C31G, or SDS. TC75
were determined from data illustrated in Fig. 3A and B. Primary human
vaginal keratinocytes were exposed to N-9, C31G, or SDS for 2, 8, 16, 24, or 48 h. At the end of each exposure interval, cell survival
was assessed by an MTT assay. The cell viability following microbicide
exposure is expressed as the fraction of viable cells relative to the
number of mock-exposed cells. The results illustrated are averages from
two experiments in which triplicate wells for each concentration were
assayed.
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In a similar experiment, primary vaginal keratinocytes were exposed
continuously to identical concentrations of N-9, C31G,
or SDS
(1.25 × 10
3%) for up to 48 h (Fig.
7). Earlier experiments (Fig.
3A)
demonstrated
that a 48-h exposure to each microbicide at this
concentration
resulted in less than 10% cell survival. After 16 h
of continuous
N-9 exposure at this concentration, cell survival
remained generally
constant between 83 and 69%. However, by 24 h,
cell viability
in the presence of N-9 fell dramatically to 8%. In
contrast, there
was no abrupt drop in cell survival during exposure to
SDS. The
decrease in cell viability associated with SDS exposure was
approximately
linear over 48 h, decreasing from 96% viability at
2 h to 7% viability
at 48 h. At 2 and 8 h, cell
survival during exposure to C31G was
at 42 and 52%, respectively. Like
the results illustrated in Fig.
6, cell survival 16 h after the
introduction of C31G decreased
abruptly (to approximately 10%).
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FIG. 7.
Microbicide toxicity increases with continued exposure
to equal concentrations of N-9, C31G, or SDS. Primary human vaginal
keratinocytes were exposed to 1.25 × 103% N-9,
C31G, or SDS for 2, 8, 16, 24, or 48 h. At the end of each
exposure interval, cell survival was assessed by an MTT assay. Cell
viability following microbicide exposure is expressed as the fraction
of viable cells relative to the number of mock-exposed cells. The
results illustrated are averages from two experiments in which
triplicate wells for each concentration were assayed.
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DISCUSSION |
The studies presented above represent one of the most extensive
uses of primary cell populations of human vaginal keratinocytes in
assessments of in vitro microbicide cytotoxicity. The effect of
microbicides on primary vaginal keratinocyte viability is highly relevant to clinical microbicide tolerance, since vaginal epithelial cells form part of the physical barrier that may impede the passage of
cell-free or cell-associated HIV-1 into subepithelial tissues (23). Microbicidal agents that compromise this barrier may
increase the risk of HIV-1 transmission.
One of the principal observations of these studies was that N-9 was
10-fold more toxic than C31G or SDS in long-term experiments using
primary vaginal keratinocytes. This observation may be particularly relevant to considerations of long-term toxicity during N-9 use. A
clinical study of N-9 retention following vaginal insertion of a
contraceptive film containing N-9 demonstrated that levels of N-9
recovered by vaginal lavage remained constant for up to 2 h after
product insertion and decreased to under 50% after 4 h
(14). A similar report described levels of retention between 19 and 7% after 2 h, detectable levels of N-9 as long as 24 h after insertion, and levels of retention dependent on the
contraceptive formulation (26). The toxicity of N-9 at low
concentrations illustrated in our long-term (48 h) in vitro experiments
(Fig. 3B) and the extended retention of N-9 observed in clinical
studies suggest that use of products containing N-9 may result in
greater levels of toxicity for longer durations following product
insertion compared to products containing either C31G or SDS.
Experiments which examined the time-dependent accumulation of
cytotoxicity emphasized differences between microbicides that may be
related to each agent's mechanism of activity. In both experiments
(Fig. 6 and 7), the time-dependent reductions in cell viability were
highly divergent, despite nearly identical levels of cytotoxicity at
the 48-h endpoint. These results suggest differences in the mechanisms
by which N-9, C31G, and SDS kill cells. The delayed reductions in cell
survival during N-9 or SDS exposure (Fig. 6) are also interesting and
suggest more complex mechanisms of cell death. Perhaps while a small
number of cells are killed quickly, most survive the first 24 h,
accumulating damage in their cell membranes. Once cell integrity is
compromised beyond a certain threshold, cells may die at a considerably
faster rate. Although C31G appears to act similarly, its higher
cytotoxicity under these conditions may result from reaching its
threshold sooner after exposure. A similar effect may account for the
higher sensitivity of primary vaginal keratinocytes to C31G during
repeated exposure (Fig. 4). These findings, which will be addressed in
future investigations, stress the need for examining not only
experimental endpoints but also intermediate exposure times when
evaluating microbicide formulations for cytotoxicity.
Examination of time-dependent cytotoxicity also highlighted the
relationship between microbicide concentration and duration of
exposure. Previous in vitro studies indicated that Escherichia coli (13) and sperm cells (25) were killed
by C31G in less than 10 s. These experiments were performed using
C31G concentrations of 2 × 102 and 5 × 102%, respectively. In studies with SupT1 T lymphocytes,
complete cell killing was achieved after 10 min at C31G concentrations above 1.25 × 102% (9). In contrast, the
results illustrated in Fig. 7, which demonstrated that a 16-h exposure
was required to reduce cell viability to 10%, were obtained using a
C31G concentration that was 16- to 40-fold lower than those used to
kill bacteria (13) or sperm (25) and at least
10-fold lower than the concentration that was completely toxic to SupT1
cells (9). These results demonstrate that in vitro
cytotoxicity is a function not only of concentration but also of
exposure duration.
At low microbicide concentrations, differences in cytotoxicity are
revealed that are otherwise masked at higher concentrations. For
example, during extended exposure (48 h), C31G and SDS were as
cytotoxic as N-9 at 5 × 103% but dramatically less
cytotoxic than N-9 at a 20-fold-lower concentration (2.5 × 104%) (Fig. 3A). Although microbicide formulations
intended for in vivo use contain active ingredients exceeding 1%,
local concentrations at the vaginal epithelial cell membrane may be far
less than in the original product due to dilution in cervical and
vaginal secretions and semen, uneven product distribution across the
vaginal epithelium, product redistribution by movement during
intercourse and normal activities, diffusion across a keratin and cell
gradient, and postapplication product loss. At these locally low
concentrations, differences in cellular sensitivity to the active
ingredient may become important. Because of its persistent cytotoxicity
at low concentration, the adverse effects of N-9 on the vaginal
epithelium may persist long after the effects of other products with
less cytotoxic ingredients, such as C31G or SDS. To determine the
relevance of low concentration differences in cytotoxicity to in vivo
microbicide use, studies of product distribution and retention will be
necessary to complement in vitro examinations of microbicide
cytotoxicity and activity.
Studies of sensitivity to microbicide exposure performed with primary
vaginal keratinocytes presage ongoing efforts to examine the effect of
elements within the vaginal milieu on microbicide efficacy. In vitro
assays described in this manuscript can provide assessments of
potential activity and cytotoxicity relative to other agents, but they
are not suited to accurately reflect the in vivo value of a
microbicide, measured in terms of both microbicidal activity and its
effect on cell viability. More complete models would take into account
additional factors relevant to the vaginal microenvironment, including
the presence of vaginal and cervical secretions, changes in pH,
osmolarity, and protein content, the influx of semen during
intercourse, the architecture of the vaginal epithelium, and
time-dependent reductions in product retention (14). These
factors may independently affect the in vivo activity and cytotoxicity
of a given agent and change the concentrations at which these
properties are manifested. We presume that these in vivo factors will
decrease cytotoxicity associated with microbicide application and
increase the effective antimicrobial activity of the microbicidal
agent. Although animal models (16) and clinical trials may
offer more complete experimental conditions, in vitro experiments have
the advantage of convenience, flexibility, speed, and low cost. Ongoing
investigations of vaginal microenvironmental factors are now focused on
the influence of protein on microbicide activity. Proteins and mucins
within the vaginal and cervical mucus may serve to sequester surfactant
microbicides, lessening their effective concentrations and their
interactions with STD pathogens and the surrounding tissues. This may
be especially true of protein sequestration of SDS, which binds with
high affinity to proteins.
These investigations have served to advance our understanding of
microbicidal toxicity. First, surface-active agents like N-9, C31G, and
SDS may function as microbicides using distinctly different mechanisms,
as suggested by the divergence in cellular sensitivity during long- and
short-term exposure. Additionally, SDS, which is well-known for its
ability to denature proteins, may function as a protein denaturant at
low concentrations and as a surfactant at higher concentrations.
Understanding the different mechanisms by which these agents act may
facilitate the design of more effective microbicides with broader
activity and lower cytotoxicity. Future experimentation will explore
these and other aspects of microbicide cytotoxicity. Second, these
studies have provided the foundation upon which in vitro models of the
vaginal microenvironment can be constructed to explore the impact of
factors such as pH and the epithelial architecture on microbicide
efficacy. Efforts are being directed toward constructing in vitro
vaginal microenvironment models that would more closely emulate the
conditions within the vagina and allow questions of in vivo efficacy to
be better addressed.
In vitro experiments regarding antiviral potential as well as
cytotoxicity have implied that C31G and SDS may be attractive alternatives to N-9 as topical vaginal microbicides (9). The present studies, which demonstrate high N-9 cytotoxicity, reinforce the
concept that C31G and SDS may be desirable alternatives to N-9. These
in vitro experiments will be complemented by ongoing investigations
exploring the efficacy of potential vaginal microbicides, including
C31G and SDS, using a human vaginal epithelial xenograft system in
immunocompromised mice (6). Both approaches will advance the
characterization and formulation of these potential vaginal
microbicides and provide the foundation for additional human trials.
| |
ACKNOWLEDGMENT |
These studies, performed in the laboratories of B.W. and M.K.H.,
were supported by Public Health Service grant P01 AI37829.
| |
FOOTNOTES |
*
Corresponding author. Mailing address: Department of
Microbiology and Immunology (H107), The Pennsylvania State University, College of Medicine, 500 University Drive, P.O. Box 850, Hershey, PA
17033. Phone: (717) 531-8258. Fax: (717) 531-5580. E-mail: bwigdahl{at}psu.edu.
| |
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Antimicrobial Agents and Chemotherapy, July 2000, p. 1954-1960, Vol. 44, No. 7
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Top
Abstract
Introduction
