TRANSCRIPT for Webinar with the title: Herpes simplex virus (HSV) diagnostics 2025: An overview
0:02
Hello everyone.
0:03
Welcome to our webinar on herpes simplex diagnostics.
0:06
My name is Bob Jones and I'm the Medical, the moderator for today's session and the
0:10
Senior Medical Director for Infectious Disease at Quest Diagnostics.
0:14
I've been with Quest for over 8 years after spending 25 years in clinical
0:19
infectious disease practice.
0:21
We have two outstanding speakers today who will review the current state of
0:26
herpes simplex virus diagnostics.
0:29
Our first speaker is Dr Beth Marlowe.
0:31
Beth is the Executive Scientific Director and leads research and development for
0:36
Quest Diagnostics, Infectious Diseases and Immunology.
0:39
She received her PhD from the University of Arizona followed by a postdoctoral
0:45
fellowship at UCLA.
0:47
Before joining the team at Quest, she worked for Genpro Kaiser Permanente
0:51
and held the position of Global Director of Medical Affairs at Roche Molecular
0:57
Systems.
0:57
She's a diplomat of the American Board of Medical Microbiology and has served on
1:03
several editorial boards.
1:06
Our second speaker is Dr Susan Realegeno.
1:10
She's currently a scientific director at Quest Diagnostics in San Juan Capistrano,
1:15
CA in the infectious diseases department.
1:18
She obtained her PhD from UCLA in microbiology,
1:21
immunology and molecular genetics and completed her clinical microbiology
1:26
fellowship at UCLA.
1:28
Susan is board certified in medical microbiology and currently overseas
1:33
serology testing and supports areas of molecular testing and research and
1:38
development at Quest Diagnostics.
1:42
Thank you, ladies, and looking forward to a great
1:44
conversation.
1:47
Thank you, Dr Jones, for that gracious introduction.
1:54
Thank you for attending our webinar today.
1:57
The objectives of our webinar today are to provide an overview of herpes simplex
2:03
virus or HSV, review the testing that's available for
2:07
HSV, highlight the current landscape for HSV
2:10
testing as well as diagnostic considerations for genital herpes as
2:15
outlined in the CDC guidelines, and discuss the diagnostic limitations
2:20
around that testing.
2:27
Herpes simplex virus is a member of the herpesviridae family.
2:32
There are 9 herpes virus types that are known to primarily infect humans,
2:36
and at least five of those are widespread among humans.
2:41
Herpes simplex virus 1 and herpes simplex virus 2 are the focus of today's talk.
2:46
HSV is the leading cause of genital ulcer disease worldwide,
2:51
predominantly due to HSV-2 and to a lesser extent, HSV-1.
2:57
It can cause chronic, lifelong latent infection with
3:00
asymptomatic or symptomatic reinfection.
3:03
As illustrated on the slide, these are large, enveloped,
3:07
double stranded DNA viruses.
3:10
The envelope makes up the outermost part of HSV and consists of a lipid bilayer
3:15
membrane which is studied with an array of 12 distinct types glycoproteins.
3:22
The glycoproteins are required for viral entry and elicit neutralizing antibodies.
3:27
It's the differences in glycoprotein G between HSV-1 and HSV-2 that have been
3:33
utilized in the development of HSV type specific serologic assays that Dr
3:38
Realegeno will be discussing later in the talk.
3:44
HSV-1 mostly spreads through oral contact and can cause infections around the mouth
3:49
such as cold sores, or it can cause genital herpes,
3:52
which we've seen an uptick of in the last few years due to changes in sexual
3:56
behavior.
3:58
HSV-2 spreads through sexual contact and causes genital herpes.
4:09
Let's take a look at the epidemiology of HSV according to the WHO.
4:14
Globally, an estimated 3. 8 billion people under the age of 50 have
4:19
HSV-1 infection, the main cause of oral herpes,
4:23
while an estimated 520 million people between the ages of 15 and 49 worldwide
4:29
have HSV-2 infection, the main cause of genital herpes.
4:34
Most HSV infections are asymptomatic or unrecognized.
4:39
Symptoms of herpes include painful blisters that can occur over time.
4:43
Genital herpes is among one of the most prevalent sexually transmitted diseases
4:47
in the United States.
4:49
Although both HSV-1 and HSV-2 can potentially cause genital infection,
4:54
most causes of genital herpes in the US are caused by HSV-2.
5:00
In 2018, there was an estimated 18. 6 million people between the ages of 18
5:05
and 49 years of age living with genital herpes caused by HSV-2,
5:10
an additional several millions others living with HSV.
5:16
In 2018 alone, it was estimated that almost 600,
5:19
000 persons 18 to 49 years of age had newly acquired HSV-2 infections in the
5:23
United States.
5:25
Since genital herpes is not a nationally notifiable condition,
5:29
the true prevalence of persons living with genital herpes and incidents of new
5:33
cases is difficult to determine.
5:36
The best seroprevalence data in the US is through the NHANES or National Health and
5:41
Nutrition Examination Survey.
5:44
Based on this data, which was collected between 2015 2016,
5:49
the prevalence rate was estimated at 12. 1%.
5:55
As you see from the graph, there's been a significant decline in
6:00
HSV-2 seroprevalence trends from 1999 - 2000,
6:04
where it was 18% to the more recent estimates of 12%.
6:09
Of note are the HSV-2 differences in gender,
6:13
where prevalences were nearly twofold higher among females compared to males.
6:20
As expected, seroprevalence notably increases with age
6:24
and disparities have been identified in HSV-2 prevalent rates with the highest
6:29
rates in non Hispanic black individuals and these disparities were persistence
6:33
among the time frames.
6:35
As seen in the graph, the clinical manifestations of genital
6:41
herpes vary significantly when comparing first clinical episodes and recurrent
6:50
outbreaks.
6:52
The severity, frequency of clinical manifestations,
6:56
and recurrence rates are influenced by the virus type as well as the immune
7:02
status of the host.
7:05
Persons who are serial positive for HSV-2 and not aware of their genital infection
7:10
account for the majority of genital HSV infections.
7:14
Initial HSV-2 genital infections in persons with a previous HSV-1 antibodies
7:20
are often asymptomatic.
7:23
Approximately 80% of people positive for HSV-2 have never received a diagnosis for
7:31
genital HSV evaluation.
7:33
Of people who have been undiagnosed with genitals,
7:37
HSV-2 have demonstrated that an estimated 20% have true asymptomatic infection or
7:43
they have a current of genital lesions and locations that maybe were not easily
7:49
identified, such as on the cervix.
7:53
The remaining 60% have mild, unrecognized symptoms.
7:58
Additionally, some symptoms caused by HSV may be
8:00
mistaken for other disorders such as vaginitis, hemorrhoids,
8:03
or allergic reactions.
8:06
When asymptomatic, HSV-2 seropositive individuals receive
8:10
education about the merit of symptoms caused by genital HSV infections.
8:15
It's been reported that approximately 2/3 will subsequently identify symptoms that
8:21
are consistent with genital HSV-2 infection.
8:30
The first clinical episode of HSV refers to the initial symptomatic occurrence of
8:35
herpes.
8:36
This can be an ulcer either on the oral, pharynx, skin, or genital mucosa.
8:42
Primary infection is defined as the first infection with either HSV-1 or HSV-2,
8:46
with the absence of antibodies to either.
8:50
Symptoms include bilateral genital ulcers, ulcers which are painful, itching,
8:56
dysphoria with vaginal or urethral discharge,
9:00
and tender equinal adenopathy without antiviral therapy.
9:05
Lesions can last two to three weeks with the evolution of lesions from a vascular
9:11
pustule to wet ulcers to dry crust.
9:14
Recurrent symptomatic herpes refers to the recurrence in a setting of known
9:20
diagnosis of genital HSVs.
9:23
This can happen with oral HSV.
9:26
Recurrent symptoms are characterized by mild localized symptoms that typically
9:31
resolve within two to five days after onset of prodromal symptoms like
9:36
localized tingling or burning due to HSV traveling along the nerve axons.
9:42
That's This is common and begins typically 12 to 24 hours before the 1st
9:46
lesions appear.
9:51
The frequency of symptomatic genital herpes reactivation to HSV-2 decreases
9:56
from a medium of four to five recurrences for the first year to three to four
10:01
recurrence in subsequent years.
10:04
For genital HSV-1.
10:05
The frequency of symptomatic genital herpes is a medium of one year,
10:09
one per year during the first year, and typically no outbreaks are seen in
10:14
subsequent years.
10:16
Reactive symptomatic infection is higher in women than in men and in persons who
10:21
experience prolonged symptoms associated with primary infection.
10:26
There are complications of HSV infection, and this includes karyentitis and social
10:31
nervous infections.
10:32
CNS infections, such as a aseptic meningitis,
10:35
account for approximately 10% of all cases of aseptic meningitis,
10:40
with most cases caused by HSV-2 infection.
10:45
HSV encephalitis is typically caused by HSV-1.
10:49
Uncommon complications of HSV include benign recurrent lymphatic meningitis,
10:55
also known as Mollaret's meningitis.
10:59
Neonatal HSV infection can also occur and is defined as HSV infection that develops
11:06
in a newborn during the first 28 days after birth.
11:11
It is a rare complication and occurs in about one in 3000 deliveries in the US.
11:16
The risk of transmission is highest in persons who acquire primary genital
11:20
herpes infection at or near the time of delivery.
11:24
Among neonatal transmission, 85% occur at delivery, 5% in utero,
11:30
and 10% postpartum.
11:35
Transmission of HSV usually occurs through close contact and direct contact
11:41
with people who are shedding virus at the mucosal or epithelial surface or in
11:46
genital or oral secretions.
11:50
The transmission of HSV too often involves asymptomatic shedding of the
11:56
virus in a person unaware that they have HSV.
12:00
As discussed earlier, HSV can be transmitted perinatally from
12:04
mother to child at the time of delivery, and fomite transmission of HSV is
12:10
unlikely, although auto inoculation can occur due
12:13
to viral particles from genital sites or other eucocutaneous sites from fingers,
12:19
usually during primary infection.
12:25
Clinical diagnosis of HSV can be challenging because many people are
12:30
asymptomatic and undiagnosed.
12:33
The clinical diagnosis of genital herpes should be confirmed by laboratory testing.
12:38
This slide is an overview of the generally available diagnostic test.
12:43
Diagnostics include molecular techniques such as PCR, cell culture, serology,
12:50
antigen detection and cytology.
12:54
The recommended test for direct detection of HSV and clinical symptoms samples are
13:00
molecular assays or cell culture.
13:03
Molecular methods are the most sensitive method of the two.
13:07
For serology, a 2-step type specific serology is
13:11
recommended for detecting antibodies while antigen and cytology methods are
13:16
not recommended due to low sensitivity.
13:19
Dr Realegeno
13:21
will go into further detail about the recommended diagnostics in the second
13:25
half of this webinar.
13:29
In terms of prevention and treatment, today there are no vaccines against HSV-1
13:35
or HSV-2.
13:36
Prevention includes minimizing close contact,
13:38
especially when lesions are present.
13:41
People should make sure that they practice good hygiene and wash their
13:44
hands and don't touch their eyes or mucosal area if they are infected.
13:48
If intercourse is involved, barrier protection is recommended and
13:52
caesarean delivery for mothers with active lesions.
13:56
There is antiviral treatment that's available for HSV.
14:00
HSV antiviral therapy includes 3 available nucleoside analog medications,
14:06
acyclovir, galicyclovir, and famciclovir.
14:11
Oral therapy is recommended when lesions occur,
14:14
and IV acyclovir treatment is available for more invasive infections,
14:18
such as those seen with central nervous infections or neonatal infections.
14:24
HSV may become resistant to first line and second line treatments,
14:27
although treatment susceptibility testing may be useful to help guide treatment
14:32
when patients aren't responding to medications.
14:35
This testing is available by phenotypic or genotypic susceptibility testing and
14:40
available through reference laboratories.
14:44
The history of HSV in acyclovir therapy is an interesting one if you've ever read
14:50
Ina Park's book Strange Bedfellows, which I highly recommend if you're
14:55
interested in a fascinating trip down history around STIs.
15:00
Is in 1982, the first FDA approved approval for
15:04
acyclovir became available and this was an acyclovir ointment for the treatment
15:10
of genital herpes.
15:12
It was a first of its kind antiviral drug able to suppress the virus but not
15:17
eradicate it and it later served as a prototype for antiviral drug development
15:21
against HIV.
15:24
Ironically, the marketing department predicted that
15:26
the sales of acyclovir would be modest and peak at about 10 million a year.
15:31
Well, this might seem like a good return on
15:32
investment.
15:33
It really dwarfed in comparison to other blockbuster drugs at the time like Zantac,
15:38
which had annual sales of $2 billion.
15:41
Ironically, it was a Time magazine article that
15:44
unexpectedly helped the cause around the uptake of acyclovir in August 1982 when
15:49
Time published a story entitled Today's Scarlet Letter with a giant H across the
15:54
cover of the magazine.
15:57
While Time never mentioned acyclovir or its manufacturer,
16:00
the public awareness of herpes grew as well as the interest in herpes treatment
16:04
and acyclovir was the only product on the market.
16:07
As a result, the media interest rose and from 1982 to
16:12
83, more than 1000 news articles were written
16:15
about the drug manufacturer and acyclovir.
16:19
Now this is really fascinating if you think about the fact that this was before
16:23
the age of digital communication.
16:25
Everything was still in print.
16:28
The ointment formulation of acyclovir was only approved for initials herpes
16:32
outbreaks and only reduced pain from outbreaks in men.
16:36
Acyclovir was later formulated into a capsule to be taken orally and speed up
16:40
the healing sores of initial infections and recurrent outbreaks.
16:45
By the end of January 1985, the FDA approved acyclovir capsules for
16:49
both men and women with herpes to be used for initial and recurrent outbreaks.
16:55
This was also around the time that direct consumer marketing was in its infancy.
17:00
The FDA did not explicitly forbid it, but it did call for a voluntary
17:04
moratorium on the practice between 83 and 85.
17:08
However, by 1986, the FDA lifted that moratorium and a
17:11
series of ads are run, which, by the way, had no mention of the product acyclovir
17:17
or the claims for the drug.
17:19
The ads increase attention to the disease and encourage consumers to get medical
17:23
attention.
17:24
Despite the subtlety of the ads of acyclovir capsules were just a big
17:28
success and shattered all previous predictions of sales and they reached
17:32
over 1 billion annually and eventually accounted for 1/3 of Burroughs welcomes
17:37
sales and half of its operating profits.
17:40
One of the pharmacologist Trudy Elion, was awarded the Nobel Prize in 1988 due
17:46
in part to the discovery of acyclovir.
17:49
The process.
17:50
The success of the drug later caught the attention of the pharmaceutical giant
17:55
Glaxo, which was acquired by the company in 85
17:57
for $14 billion.
18:00
Simultaneously, improvements in diagnostic testing were
18:03
occurring, which were allowing more diagnosis to be
18:06
made.
18:07
In the early 1980's, the diagnosis of herpes could only be
18:10
confirmed with viral culture as well as other direct methods such as DFA
18:15
techniques to detect HSV from active lesions.
18:19
This meant that only patients who had active symptoms could be certain of
18:23
diagnosis.
18:25
By the end of the 80's, the first herpes antibody test,
18:28
which could distinguish HSV-1 and HSV-2, began to hit the market and allowed
18:32
patients to begin to get blood tests regardless of the symptoms.
18:38
As we discussed earlier, undiagnosed, undiagnosed HSV makes up the large
18:43
portion of HSV infection due to asymptomatic and undiagnosed infection.
18:48
Today in 2026, we continue to see an evolution of
18:53
clinical diagnostics for HSV.
18:56
It's pretty amazing when you think about the fact that HSV has been overshadowed
19:01
for years by other STI's like syphilis and gonorrhea.
19:05
It wasn't even mentioned in the best selling sexual manuals in the 60s that
19:09
discussed venereal diseases.
19:11
In the 1977 VD handbook, which would by the way was a Canadian
19:16
manual, it devoted 14 pages to gonorrhea and two
19:19
to genital herpes.
19:21
Despite humans living with strains of HSV for hundreds of thousands of years and
19:26
descriptions of genital herpes appearing in scientific writing starting around
19:31
1736, the lack of attention was attributed to
19:34
the lack of treatment options for people with a diagnosis.
19:38
I think this further highlights the importance of having available
19:42
appropriate diagnostic testing.
19:44
And with that, I will hand it over to Dr Susan Realegeno
19:47
who will provide a more in-depth discussion of HSV diagnostics that are
19:51
available today.
19:53
Thank you, Dr Marlowe for that great introduction
19:56
and interesting history behind HSV.
19:58
It really brings attention to how important this infection is and why we're
20:03
talking about it.
20:04
So in this part of the talk, I'm going to focus on laboratory testing
20:08
like Dr Marlowe mentioned, and then I'll further go into utilization.
20:12
Limitations of certain types of testing, especially serological methods that are
20:17
used for genital herpes.
20:20
A diagnosis of HSV infection can be achieved through clinical evaluation and
20:24
further confirmed with laboratory testing using an appropriate specimen type.
20:29
So there are direct and indirect methods including biological tests and antibody
20:33
detection assays respectively.
20:36
These the type specific nucleic acid amplification tests such as PCR or TMA
20:41
are the most sensitive and preferred method for detection of HSV during acute
20:46
infection and also in patients with recurrent symptomatic infection.
20:51
There are other methods but they have lower sensitivity and that includes viral
20:56
culture and they may require additional testing for HSV specific typing.
21:01
Viral culture is also needed if phenotypic antiviral susceptibility
21:05
testing is performed.
21:07
Antigen and cytology examination overall also have lower sensitivity and are not
21:12
recommended for direct detection, but they may still be available at
21:16
certain institutions.
21:17
Finally, we have antibody detection tests which
21:21
include type specific HSV-1 and HSV-2 IgG test.
21:24
They may be used to help evaluate previous exposure.
21:28
However, serological testing when supporting
21:31
diagnosis of genital herpes is not recommended as a primary method,
21:35
but is recommended in certain scenarios due to the analytical limitations of
21:40
currently available methodologies.
21:47
When looking at the different clinical manifestations and what the preferred
21:52
laboratory method for confirming infection,
21:55
HSV NAAT is preferred across the board with several manifestations including
22:00
neonatal herpes, which requires a swab of multiple sites,
22:03
CNS infection, ocular involvement, and genital or herpes.
22:08
Collecting the appropriate specimen type is really important to ensure that you
22:12
have high sensitivity and specificity for these tests.
22:15
Viral culture is still listed in the guidelines as one of the acceptable
22:20
methods for recovering HSV from surface specimens and neonatal infection,
22:25
but it's not recommended for CSF due to the low viral yield and the risk of false
22:30
positives.
22:31
Genital herpes, in addition to having NAAT as the
22:35
preferred method for laboratory diagnosis, also include serological testing when
22:40
there are no lesions present.
22:46
Since NAATs are the preferred method for direct detection and diagnosis of herpes,
22:51
I wanted to give some examples of commercially available assays and their
22:55
intended use.
22:56
So there are several FDA cleared type specific HSV net acids that are available
23:01
and they come either as single Plex where they only contain HSV-1 and HSV-2 or they
23:06
can be found in Multiplex tests containing additional analytes.
23:11
For example, some of them may have VZV, while others may have an extensive list
23:15
of of additional analytes.
23:17
In the case of the meningitis encephalitis panels,
23:20
you'll see that the approved specimen types are limited to either cutaneous or
23:26
mucocutaneous lesions, sometimes restricted to the anogenital
23:30
region.
23:31
And then CSF samples for patients who have meningitis encephalitis or CNS
23:38
involvement.
23:40
And then these are specifically for patients who are symptomatic.
23:45
Several published studies have shown that the performance of these assays have
23:49
really high analytical sensitivity and specificity compared to other methods.
23:53
And it's important to note that random or blind swabs in the absence of lesions is
23:57
not recommended since this will decrease your clinical sensitivity and those
24:01
negative results may not rule out infection.
24:03
So that just is goes to show that you really need to use these tests
24:07
appropriately in order to have the highest clinical sensitivity and
24:12
specificity.
24:13
Some of these assays are not approved for patients under 18 years old or they
24:18
explicitly state that they're not for prenatal testing or I mean prenatal
24:23
screening.
24:23
So it's really important to know what test your platform you're using and what
24:27
the limitations are for those for those platforms and the instructions for use.
24:31
There are also additional qualitative and quantitative laboratory developed tests
24:36
that are available through commercial laboratories and these are used to
24:40
accommodate testing for additional specimen types that might not be FDA
24:45
cleared or for specific conditions that go beyond your typical HSV manifestations.
24:50
And some of those specimen types that are off label or are tested with LD TS might
24:56
include whole blood, serum, plasma tissue, maybe ocular fluid and they may not be
25:02
widely available.
25:08
Now I'm going to shift over to talking about type specific serological tests and
25:12
their performance characteristics specifically in the context of genital
25:16
herpes since I think this is a really important topic like Dr Marlowe had
25:20
highlighted previously.
25:22
So there's a variety of serological testing methods that are available and
25:26
used to support diagnosis or seroprevalence studies.
25:30
And these include type specific antibody assays that differentiate HSV-1 and HSV-2
25:35
antibodies using glycoproteins G1 and G2 as a target antigens.
25:41
Common commercially available methodologies include chemoluminescence
25:45
amino assays, which are really large platforms that are
25:48
FDA cleared that can accommodate high throughput testing.
25:52
There's also your traditional enzyme linked immunosorben assays, the ELISA.
25:57
There's electrochemoluminescence, amino assays, Multiplex flow immunoassays,
26:02
lateral flow, which come in point of care formats and
26:06
amino blot assays that could all be purchased from manufacturers and are FDA
26:11
cleared and vary in terms of of their complexity.
26:15
Western blot is considered the gold standard and many of these platforms have
26:20
been compared to Western blot.
26:22
And I'm going to go over a little more detail about some of these assays in
26:25
other slides.
26:27
One other important note that I want to make is that HSV IgM testing is no longer
26:33
available and that is because these assays lack the sensitivity to be used as
26:39
a reliable marker for active infection.
26:43
IgM antibodies, they can persist for months following
26:46
primary infection or they may or may not develop when you have recurrent infection,
26:51
whereas IgG will persist indefinitely.
26:53
So therefore IgM is is not is not something that you you want to use for
27:00
diagnosing acute or active infection.
27:07
When interpreting qualitative results from a HSV serological test,
27:11
there are certain limitations that need to be considered.
27:14
Since HSV-2 infections are usually sexually acquired,
27:18
the presence of HSV-2 IgG antibodies can indicate an anogenital herpes infection.
27:24
However, in contrast, the presence of IgG of IgG HSV-1 cannot
27:29
be used to support a genital herpes diagnosis.
27:32
Since HSV-1 infections are not limited to the anogenital region and can be acquired
27:38
during childhood so that one has limited utility when it comes to diagnosing
27:44
genital herpes.
27:46
Also, seroconversion can occur between two
27:49
weeks and three months with the majority of patients developing antibodies by 12
27:53
weeks.
27:53
So detection of if of antibodies can be also delayed in certain patients.
27:59
So knowing the that a negative result does not rule out infection.
28:04
If you recently suspect acquisition to be within that window,
28:08
then follow up testing may be indicated to to observe that sero conversion,
28:13
especially if it's recent recent infection.
28:18
And then detection of seroconversion can also vary depending on the type of method
28:22
or platform that you're using because they might they might have different
28:26
clinical sensitivities and I'll mention that in another slide.
28:34
So when is HSV serological testing indicated when being used for genital
28:40
herpes?
28:41
So the 2021 CDC STI Treatment Guidelines state that if a lesion is present,
28:46
then you want to swab that lesion and testing should be performed using a type
28:51
specific nucleic acid amplification test or viral cultures.
28:55
But what happens when you don't have a lesion present and you're still
28:59
suspecting genital herpes?
29:00
Well, the guidelines say that HSV-2 antibody
29:04
testing for IgG can be used, but only are under specific scenarios.
29:09
So those scenarios include if a patient has recurrent or atypical genital
29:15
symptoms or the lesion, you did swab A lesion and send it for
29:20
NAAT testing, but it comes back negative by either NAAT
29:25
or culture.
29:26
Or you have a person with a clinical diagnosis of genital herpes but without
29:30
any laboratory confirmation.
29:33
Or if you have a patient that's at higher risk for infection and for example,
29:38
one who has had a partner who has been diagnosed with genital herpes,
29:43
or if somebody is presenting for an STI evaluation,
29:46
those would be cases where HSV serological testing may be indicated.
29:56
When reviewing the US Preventative Services Task Force recommendations
30:01
specifically for screening that in conjunction with the CDC STI Treatment
30:07
Guidelines, both say that routine screening for a
30:10
genital HSV infection and asymptomatic individuals,
30:14
including pregnant women is not recommended.
30:18
This is due to the low specificity and high likelihood of false positives of
30:23
certain currently available assays when used for population based screenings,
30:28
which can lead to more harm than good in these in these patients.
30:33
Therefore, screening is not indicated in a person
30:36
with no known history, signs or symptoms of genital HSV
30:39
infection, including those with unrecognized
30:42
infection.
30:43
However, those at risk of acquiring infection,
30:46
like I mentioned before, regardless of pregnancy status,
30:49
including individuals with HIV or other immunosuppressive disorders,
30:53
can still be tested.
30:59
So many of the of the studies that have informed the HSV-2 IgG testing
31:04
recommendations for genital herpes have been using the HSV-2 IgG ELISA.
31:11
Performance characteristics such as sensitivities and specificities can vary
31:16
widely depending on the patient population tested,
31:19
the prevalence of that patient population, the timing of specimen collection,
31:24
and what the reference standard was used to characterize what a true positive is.
31:29
For example, some studies have shown a range of 80 to
31:34
98% for sensitivity and 57 to 98% for for specificity.
31:40
There have been also a number of studies that have shown poor specificity using
31:46
the ELISA and focusing on that lower range and showing that false positives
31:51
can occur more frequently at lower index values, specifically between 1.1 and 3.0.
31:58
More recently, there has been more published studies
32:03
using the FDA cleared more updated platforms.
32:07
And there's one study published by Dr Harry Prince,
32:10
actually 2 studies that compared the ELISA to the chemoluminescence platform,
32:16
which I refer to as CIA in these slides.
32:19
What these studies showed was that the discrepant result that there were
32:24
discrepant results between these two platforms and that false positives
32:28
actually can occur throughout the entire index range of the assay,
32:32
not just between 1.1 and 3.0.
32:34
For example, when looking at a cohort of over 2000 CIA
32:38
positive samples, 18% of them had ELISA negative results.
32:43
If you look at the breakdown by index value of those discordant results,
32:49
79% of them were between 1.1 and 3.0, and collectively 96% of the total
32:55
discordant samples were between 1.1 and 6. 0.
33:00
Conversely, when looking at the concordance samples
33:03
where both the CIA and the ELISA are positive,
33:06
those tended to be confirmed as true positives 97% of the time.
33:11
So the discrepancies between two methodologies may be due to either
33:15
differences in antigen used, clinical sensitivity of the platform,
33:19
or any analytical performance characteristics.
33:26
To further highlight differences in sensitivity between two methodologies
33:30
from a clinical perspective, there was one study looking at time to
33:34
seroconversion following HSV-2 primary infection by ELISA compared to Western
33:39
blot.
33:40
In this study, they tested paired samples collected from
33:43
a cohort of patients with newly acquired HSV-2 infection,
33:47
and they showed that the median number of days to seroconversion was shorter using
33:52
the ELISA compared to the Western blot.
33:55
So by six weeks, ELISA had detected 77% of the cohort,
33:59
while Western Blot had only detected 53%.
34:03
Because positivity for the Western Blot is based on reactivity to an array of HSV
34:08
antigens, they actually looked at HSV reactivity in
34:11
samples that did not meet the criteria for to be considered positive.
34:16
And they refer to this as a limited profile.
34:19
And there they showed a higher proportion of positivity at six weeks.
34:22
And this demonstrated that there was evidence of seroconversion.
34:27
So by 6 months, Western blot was able to detect 100% of
34:31
the seroconversion and ELISA 93% in this cohort.
34:35
And then what this study demonstrates is that timing of specimen collection and
34:39
methodology used for testing is important when interpreting results depending on
34:44
what stage of the infection you're in and when evaluating data from these studies
34:48
that use Western blot as a comparator for true positives.
34:55
More recently, there was a study published in the
34:58
Journal of Clinical Microbiology actually comparing 3 automated FDA cleared
35:03
platforms for the diagnosis of genital herpes using two characterized sample
35:07
cohorts.
35:08
The first cohort consisted of remnant samples submitted for Western blot
35:12
clinical testing and the second cohort included samples collected from persons
35:17
who had been diagnosed with genital herpes by either PCR or culture at least
35:22
six months prior.
35:23
So that would indicate that they should have their sero converted by then.
35:28
Concordance between the automated platforms in Western blot range from 78%
35:34
to 95% and HSV-2 positive and 92 to 100% for HSV-2 negative samples.
35:41
In addition, concordance was higher in samples that
35:46
were HSV-2 positive, HSV-1 negative compared to samples that
35:51
were HSV-2 and HSV-1 dual positive.
35:56
Additional analysis for sensitivity and specificity using NHANES
36:00
Population prevalence rates showed an overall range of about 95 to 98%
36:06
sensitivity and a 94 to 99% specificity when looking at all the samples on all
36:12
platforms.
36:14
So although there were select platforms that had higher rates of sensitivity and
36:19
specificity for HSV-2 compared to others depending on the cohort analyzed,
36:24
overall the data shows that the current FDA cleared platforms for testing HSV-2
36:29
have relatively high concordance compared to Western blot and to each other,
36:33
and high sensitivity and specificity in detecting antibodies and individuals with
36:38
confirmed genital herpes.
36:41
However, the consensus is that there still may be
36:44
gaps in room for improvement when it comes to HSV serologic testings.
36:48
And there's a lot more data in this paper.
36:50
So I encourage you to kind of go review it because it really depends how you
36:54
interpret the data and, and, and looking at the different platforms
36:58
and then getting an overall picture of how these different platforms performed
37:03
in what kinds of samples.
37:09
Because of the risk of false positives and the potential impact it may have on
37:13
patients, the 2021 STI Treatment Guidelines
37:16
actually recommend a 2-step testing algorithm when you're using an antibody
37:20
test to support diagnosis of genital herpes.
37:24
These guidelines were largely based on studies using ELISA,
37:27
which showed that the specificity was poor for these assays,
37:30
especially at the lower index values like I mentioned before.
37:34
Therefore, it's recommended that a positive IgG
37:37
sample should be confirmed using a second test that utilizes a method that's
37:42
distinct from the initial test and has a different antigen.
37:47
The Biokit and the Western blot assays were both provided as possible
37:51
confirmatory tests in the guidelines due to several studies showing that they can
37:55
improve overall accuracy of initial HSV results.
38:03
However, there are several limitations to
38:05
performing confirmatory testing.
38:08
One of the major limitations overall is that confirmatory testing is not readily
38:12
available.
38:14
For instance, the Western blot is available only at one
38:16
institution, the University of Washington.
38:19
And although it's considered the gold standard,
38:21
it's a very technically challenging and labor intensive assay.
38:26
And like I mentioned before, if it's early infection,
38:29
it might not be as sensitive as some of the other platforms available.
38:34
There's also a point of care device that can be purchased commercially.
38:38
It has been marketed under several different names.
38:41
The most commonly recognized is the Biokit.
38:43
The advantage of this of this device is that it's rapid and it can be performed
38:47
on site without any instrumentation.
38:49
However, reading can be subjective and there have
38:52
been supply challenges from the vendor throughout the years and it's not
38:56
amenable to high throughput testing.
38:59
There's also immunoblots that are commercially available that are easier to
39:03
perform compared to the Western blot the FDA cleared.
39:07
Reading is easy and standardized.
39:08
However, these were common antigens that could
39:11
potentially be the same as some of the screening assays and therefore not always
39:15
ideal for confirmatory testing.
39:17
Lastly, there is the HSV-2 IgG inhibition assay
39:21
that's available at Quest Diagnostics.
39:25
This is a reflex test that is intended to be used to confirm screen positive
39:30
samples with index values between 1. 1 and 6.0.
39:34
However, it's only offered at Quest and
39:37
occasionally if there is a sample with low IgG levels,
39:40
the inhibition results may not be determined,
39:43
and I'll go over this in more detail in subsequent slides.
39:47
I also want to highlight that the CDC guidelines point out that when
39:51
confirmatory testing is not available, patients should be counseled about the
39:56
limitations of serological testing, including the risk of false positive
40:00
results, before proceeding with with serologic
40:02
testing.
40:08
For comparison, I just wanted to give examples of how
40:12
confirmatory methods work.
40:14
The Western blot on the left utilizes proteins from lysates of HSV infected
40:20
cells and patient.
40:21
Antibodies bind to the viral proteins and depending on the reactivity to specific
40:26
bands, HSV-1 and HSV-2 antibody detection is
40:29
determined.
40:31
The immunoblot is similar but more straightforward.
40:33
It uses recombinant antigens that can be more clearly interpreted.
40:37
It does not have the wider way of banding pattern as the Western blot does though.
40:43
Contrast.
40:43
The HSV-2 rapid test is easy to perform and can be done as a point of care test.
40:49
But like I mentioned before, reading is very subjective and may be
40:52
variable depending on the reader.
40:55
Here I gave an example that any level of reactivity is considered positive based
41:00
on the instructions for use and interpretation may be impacted by any
41:04
deviations from the manufacturer's instructions.
41:07
So it could be over calling false positives potentially depending on the
41:12
reader.
41:14
Finally, the HSV-2 IgG inhibition test.
41:17
This is an ELISA based assay that utilizes HSV-1 and HSV-2 cultural lysate
41:22
for the differential absorption of type specific antibodies.
41:26
So this allows for us to identify the presence of HSV-2 specific antibodies.
41:35
The current 2-step testing algorithm at Quest begins with an HSV-2 IgG screen
41:41
using the DiaSorin CIA platform.
41:46
Since the CDC guidelines recommend confirming samples with low indices,
41:50
specifically below 3.0, we have set the reflex criteria beyond
41:55
this range to test positive samples with an index between 1.1 and 6.
41:59
0 with the inhibition assay.
42:02
This is also supported by the data that I was previously showing that over 96% of
42:07
the discord in CIA and ELISA results are within this range using this platform.
42:13
The inhibition assay uses the HerpeSelect ELISA kit.
42:18
The assay is set up as a three-wheel assay where the patient serial is
42:22
incubated with HSV-1 culture lysate, HSV-2 cultural lysate separately and then
42:27
tested for IgG reactivity with one well to determine the baseline IgG levels.
42:33
The results are determined based on a sequential evaluation of the results.
42:38
First we ask are there any detectable IgG antibodies above the cutoff in the sample
42:43
and this is because we need a positive IgG value to actually calculate the
42:47
percent inhibition.
42:49
Therefore, negative and equivocal results do not
42:52
have an inhibition result and this is indicated by a comment on the report.
42:57
If there is detectable IgG present, we check if there's substantial
43:01
inhibition with the HSV-1 lysate.
43:04
If so, then we cannot rule out inhibition due to
43:08
HSV-1 or the lysate itself and the results is reported as indeterminate.
43:14
However, if there is no substantial inhibition
43:18
present with the HSV-1 lysate, then HSV-2 specific percent inhibition is
43:23
calculated and cut off values are used to then report positive,
43:27
which indicate a true positive screen on the CIA negative,
43:32
which indicate an initial false positive on the screen,
43:36
which is what you'll see on the report.
43:44
The HSV-2 inhibition assay has been offered at Quest Diagnostics or Focus
43:49
Diagnostics since 2002.
43:51
It was initially developed in a collaboration between Focus Diagnostics
43:55
and the University of Washington to investigate discordant results between
44:00
ELISA and Western blot in a cohort of serum from an African population.
44:06
There are there is limited data comparing the inhibition test to the Western blot,
44:11
but the original publication reported a 95% agreement between Western blot and
44:16
the inhibition assay.
44:19
They also noted that the discordant results between these two assays were
44:24
mainly from samples collected from two specific geographical regions and that
44:29
those results had low index values.
44:33
The authors also suspected that the inhibition positive Western blot
44:37
negatives may have represented early stages of seroconversion that have may
44:42
have been detected by ELISA and not Western blot.
44:47
Also atypical results that were not reported as positive by Western blot
44:51
might have been picked up by the inhibition test.
44:55
There was also one follow up study that directly compared the inhibition test to
45:01
Western blot in a African population and the overall concordance was 74%.
45:06
But similar to the original study, there are certain nuances in this patient
45:10
population that may impact the performance of the assays.
45:15
More recently, the study that I previously mentioned by
45:19
Dr Harry Prince compared over 1800 samples tested with the CIA, ELISA,
45:25
and the inhibition assay.
45:27
And then when you look at true positives, over 99% of the inhibition positive
45:32
samples were also CIA and ELISA positive.
45:36
In addition, as part of the study, the inhibition assay also demonstrated
45:40
good agreement with the biokit in samples that were CIA positive and ELISA positive.
45:47
They also looked at the breakdown of index values from the CIA screening assay
45:51
and saw that unconfirmed results tend to be at the lower indexes very similar to a
45:57
lot of the published studies with the ELISAs.
46:00
And as the index value of the screen increases,
46:05
you have you're less likely to get a discrepant result or a false positive on
46:14
the ELISA and the inhibition assay.
46:18
To summarize the key points of this talk, we have several methodologies that are
46:24
available for HSV diagnosis and that is the preferred method for lesion swabs and
46:29
CSF.
46:30
However, when there is no lesion swabs, there are recommendations for using
46:35
serological testing.
46:36
However, serological screening is not recommended
46:39
in asymptomatic individuals and with no previous history of genital herpes and
46:44
that includes pregnant women due to the the risk of false positives in some of
46:49
these commercially available platforms.
46:52
There have been published studies that shown a range of performance depending on
46:58
the methodology and patient population for HSV-2, IgG assays,
47:02
and diagnosing genital herpes.
47:04
Some of these assay may yield false positive results especially at those low
47:08
indices, which is why confirmatory testing is
47:10
currently recommended.
47:12
However, testing options are limited for
47:15
confirmatory tests and the results can depend on timing,
47:20
methodology and pre-test probability.
47:24
Additional studies to compare the performance of newer automated platforms
47:29
are starting to emerge and starting to be compared to each other and older
47:34
methodologies.
47:36
But we do need additional studies for confirmatory tests and showing how they
47:40
can be used for how good they are in diagnosing genital herpes.
47:46
Most importantly I think is that appropriate diagnostic stewardship is
47:51
required for how these tests are utilized.
47:54
We want to ensure that the assays are being used in the right patient
47:58
population in order to reduce that risk of false positives and that not only the
48:03
provider is educated, but that the patient really understands
48:07
the limitations of the test and what that what the results actually mean.
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