Monitoring human papillomavirus prevalence in urine samples: a review.

Human papillomavirus (HPV) is the main cause of cervical cancer, and many countries now offer vaccination against HPV to girls by way of government-funded national immunization programs. Monitoring HPV prevalence in adolescents could offer a near-term biological measure of vaccine impact, and urine sampling may be an attractive large-scale method that could be used for this purpose. Our objective was to provide an overview of the literature on HPV DNA detection in urine samples, with an emphasis on adolescents. We searched the PubMed database using the terms "HPV" and "urine" and identified 21 female and 14 male study populations in which HPV prevalence in urine samples was reported, four of which included only asymptomatic female adolescents. We provide herein an overview of the recruitment setting, age, urine sampling procedure, lesion type, HPV assay, and HPV prevalence in urine samples and other urogenital samples for the studies included in this review. In female study populations, concordance for any HPV type and type-specific concordance in paired urine and cervical samples are provided in addition to sensitivity and specificity. We concluded that few studies on HPV prevalence in urine samples have been performed in asymptomatic female adolescent populations but that urine samples may be a useful alternative to cervical samples to monitor changes in HPV prevalence in females in the post-HPV vaccination era. However, care should be taken when extrapolating HPV findings from urine samples to the cervix. In males, urine samples do not seem to be optimal for monitoring HPV prevalence due to a low human genomic DNA content and HPV DNA detection rate compared to other urogenital sites. In each situation the costs and benefits of HPV DNA detection in urine compared to alternative monitoring options should be carefully considered.

Human papillomavirus (HPV) is the main cause of cervical cancer.1,2 More than 35 HPV types have been identified in the genital tract, and HPV16 and 18 are responsible for approximately 70% of cervical cancer.3,4 Two HPV vaccines, a quadrivalent vaccine that protects against HPV6, 11, 16, and 18 and a bivalent vaccine that protects against HPV16 and 18, have been developed and approved by the United States Food and Drug Administration (FDA) for females 9–25 years and 9–26 years of age, respectively.5,6 The quadrivalent vaccine has also been approved by the FDA for males 9–26 years of age for the prevention of genital warts (caused by HPV6 and 11) and in both males and females 9–26 years of age for the prevention of precancerous anal lesions and anal cancer associated with the vaccine HPV types.7 However, in many countries the debate continues as to whether or not to offer the vaccine to boys in the framework of government-funded national immunization programs as is done for girls.8 Although the safety, immunogenicity, and efficacy of the two vaccines have been monitored closely in clinical trials,9–14 it is also necessary to monitor their impact in the general population.15 In addition to vaccine coverage and the incidence of cervical cancer and other HPV-related lesions, it is also recommended to monitor changes in HPV prevalence in the general population, particularly in females aged 15–20 years soon after initiation of sexual activity as this could offer a near-term biological measure of vaccine impact.16

HPV DNA detection in urine samples could be a viable alternative to detection in cervical samples for monitoring the impact of vaccination on overall and type-specific HPV prevalence.17,18 HPV DNA detection in urine samples is particularly attractive as a large-scale method among female adolescents as pelvic examination might not be feasible or ethically acceptable in this age group. HPV detection has also been performed in urine samples from males as well as at many urogenital sites.19 The urogenital sites most commonly sampled have been penile skin, specifically coronal sulcus and glans penis, and the urethra.20 In a recent review by Vorsters et al,17 41 published studies on HPV DNA in urine samples were evaluated with respect to factors that have an impact on HPV detection, such as urine sampling procedure, sample preparation, DNA extraction, and DNA amplification. They concluded that HPV DNA detection in urine is feasible and may become a useful tool but necessitates further improvement and standardization. In the same vein, Sehgal et al21 reviewed the pros and cons of using HPV DNA detection in urine samples for cervical cancer screening.21 One of their conclusions was that further research is needed to standardize and optimize the corresponding technology before recommending it as a mass screening tool for cervical cancer.

The aim of this literature review was to evaluate whether HPV DNA detection in urine samples would be a feasible approach for monitoring HPV prevalence in male and female adolescents in the general population. To this end, a list of relevant studies and their main characteristics, including HPV positivity in paired urine and cervical samples and their concordance is provided. Since only a few studies monitored HPV prevalence in urine samples from adolescents, we included relevant studies from older age groups as well. For details on factors that affect HPV DNA detection, such as urine sampling procedure, storage, centrifugation, DNA extraction, and assays for detection of human genomic and HPV DNA and an overview of the use of urine samples in a screening setting, we refer the reader to the reviews by Vorsters et al17 and Sehgal et al.21

Materials and methods

We used the terms “HPV” and “urine” to search the PubMed database in August 2012 for relevant literature. The identified studies were then individually evaluated to ascertain whether results on HPV prevalence in adolescents were reported. Studies in HIV-positive populations and renal allograft recipients were excluded as these patient groups have a reported increased risk of HPV infection. Studies that included paired urine and cervical samples were sought as they would allow for comparison of the presence of HPV in both samples. We therefore excluded female studies in which HPV DNA was detected in urine samples only, with the exception of the four studies including adolescents as they shed some light on the expected urinary HPV prevalence rates in this group. As few studies in asymptomatic male populations were found, we included the male populations of four studies despite the fact that they may be at greater risk of HPV infection: two studies on male partners of HPV-positive women, one on male partners of women with cervical cancer, and one on males with urethritis.

Whenever possible we extracted information on country, recruitment setting, age (range and mean), urine sampling procedure, total sample size, percentage of samples containing human genomic DNA, HPV assay used, proportion and type of cervical lesions, and availability of cervical sample. As a main result we report HPV prevalence in urine samples and cervical samples in female study populations. We also report sensitivity, ie, the probability of an HPV-positive urine sample given an HPV-positive cervical sample, and specificity, ie, the probability an HPV-negative urine sample given an HPV-negative cervical sample. Concordance for any HPV type and for HPV16 (and/or HPV18) was measured as the percentage of paired urine and cervical samples that yielded the same HPV result, ie, either both positive or both negative. In contrast, type-specific concordance (combined concordance for a group of HPV types) was measured only in the set of paired urine and cervical samples that were both positive for any HPV type. Within this smaller set of samples, type-specific concordance was calculated as the percent of paired urine and cervical samples that were positive for the same HPV type.

Results

HPV prevalence in females

Results from 21 female study populations from 17 publications that reported HPV prevalence in urine samples are summarized in Table 1. Four of these studies reported age-specific HPV prevalence in asymptomatic adolescents. Prusty et al22 and Manhart et al23 included females 18–25 years of age, while only two studies, one from Scotland by O’Leary et al24 and one from India by Hussain et al,25 included females less than 18 years of age (Figure 1 and Table 1). The HPV prevalence (any type) varied from 1.1% in the age group 11–14 years in the O’Leary et al24 study to 29.6% in the age group 20–21 years in the Manhart et al23 study. O’Leary et al24 reported the lowest percentage of samples (83.6%) containing amplifable human genomic DNA; Prusty et al22 reported the highest percentage (100%).

Table 1

Studies with human papillomavirus DNA detected in urine samples from asymptomatic adolescents (A) and in paired urine and cervical samples from symptomatic females all ages (B)

Author	Country	Recruitment setting/patient characteristics				Age, years range (mean)	Urine sampling procedure		HPV types – assays (types detected)a			Total sample size	Samples with human genomic DNA (%)	Lesions/HPV types (% lesions)		HPV positivity in urine samples (%)	HPV positivity in cervical samples (%)		Concordance (%)		Sensitivity (%)	Specificity (%)
Part A
Prusty et al22	India	Sexually naive college girls				18–25			In house L1 consensus primers (any type = –)			100	100 (100)	All/any typeAll/HPV16		6.04.0
Manhart et al23	USA	Randomly selected females from the National Longitudinal Study of Adolescent Health (Wave III)				18–25 (21.7)	Sampled at home		PCR with primers and dot blot with generic primers (any type = ≥36 types)			3741	3262 (95.8)b	All/any typeAll/HPV16		26.9c5.8c,d
O`Leary et al24	Scotland	Recruited from private and publicly funded schools.				11–14	Sampled at clinic		HPV INNO–LiPAe (any type = 27 types,			1341	1121 (83.6)	All/any typeAll/HR-HPV		1.1c0.9c,d
		Additional recruitment among early school leavers and oversampling in older age groups				15–18			HR-HPV = 18 types)					All/HPV16/18All/any typeAll/HR–HPVAll/HPV16/18		0.0c,d15.2c12.6c,d6.5c,d
Hussain et al25	India	Public school students				8–17 (14.1)	Sampled in private		PCR with MY primers (any type ≥ 36 types)				458	All/any typeAll/HPV16All/HPV18		3.32.20.4
Part B
Rymark et al33	Sweden		STD and adolescent clinic patients	Present or history of genital warts	16–21 (18.6)		After Pap with a cotton swab, urethral samples		In-house PCR (any type = five types) Type-specific concordance based on five types				24 (100)	All/any typeAll/Type-specific HPVNormal (54)CIN1 (42)CIN2 (4)	70.8f		62.5	83.3100.0		93.3		66.7
				Gynecological complains	15–21 (18.3)								25 (100)	All/any typeNormal (80)CIN1 (12)CIN2 (4)NA (4)	16.0f		12.0	96.0		100		95.5
Forslund et al29	Sweden		Colposcopy clinic referral. Suspected cytological changes		17–79 (37)		After gynecological exam without prior washing		In-house PCR (any type = –) and dot blot analysis. Type-specific concordance based on six types		512g		489 (95.5)	All/any typeAll/type-specific HPV	38.2		49.3	77.190.5		65.6		88.3
														Benign/any type (64)	24.8		32.1	78.7		55.4		89.7
														CIN 1/2/3/any type (30)	61.2		81.0	73.5		71.4		82.1
														Cancer/any type (1)	50.0		75.0	75.0		66.7		100.0
														Genital warts/any type (5)	73.9		78.3	78.3		83.3		60.0
Strauss et al37	UK		Randomly selected genitourinary clinic patients		16–57 (26)		Mid-stream urine		PCR with MY and GP primers (any type ≥ 36 types)		144		136 (94.4)	All/any type	65.4		77.9	75.7		76.4		73.3
Jacobson et al31	USA		Consecutively enrolled STD and adolescent clinic patients		11–20 (17.5)h		First-void		PCR with MY primers (any type = 34 types) and hybrid capture probe B Type-specific concordance based on six HR types		80		80 (100)	All/any typeAll/type-specific HPV	75.0		90.0	82.540.0i		81.9		87.5
														All/HPV16i	11.2		21.3	82.5		35.3		95.2
														All/HPV18	23.3		9.6	98.8		100		98.6
														Normal/any type (62)	65.3		83.7
														ASCUS/any type (19)	86.7		100
														LSIL-HSIL/any type (19)	100		100
Sellors et al34	Canada		Colposcopy clinic referral. Abnormal cytology		(31.5)		First-void urine after self-sampled vulvar and vaginal sample, but prior to cervical sampling		HC II (any type = 17 types)		245		200j (81.6)	All/any type LSIL (27) HSIL (36) ASCUS (37) Cancer (1)	34.5		62.5	41.0k
Stanczuk et al36	Zimbabwe		Invasive cancer patients at gynecological clinic		24–70 (44)h		Prior to cervical sampling		In-house PCR (any type = –)		43		35 (81.4)	All/any type All/type-specific HPV	88.6		100	88.6 71.0		88.6		83.3
														All/HPV16	54.3		65.7	77.1		73.9		93.3
														All/HPV18	11.4		14.3	85.7		40.0
Prusty et al22	India		Gynecological out-patient and family planning clinic patients. Married and sexually active. Complaints other than gynecological		18–35		Prior to cervical sampling using dry “paper smear”		In house L1 consensus primers (any type = –)		55		55 (100)	All/any type	9.1		9.1	100		55 (100)		All/any type
														All/HPV16	5.5		5.5	100				All/HPV16
Alameda et al26	Spain		Gynecological clinic patients.Women with poor gynecologic attention		28–55 (36)		Prior to cervical sampling		PCR with MY primers and papillomavirus clinical array (any type = –)		50		50 (100)	All/any type	22.0		34.0	80.0		52.9		93.9
														All/HPV16	16.0		22.0	90.0		63.6		97.4
														LSIL/any type (32)	6.3		31.3	75.0		20.0		100.0
														HSIL/any type (28) ASCUS/any type (40)	71.4 0.0		85.7 0.0	57.1		66.7
Daponte et al28	Greece		Colposcopy clinic referral. Abnormal cytology				First-void urine prior to colposcopy and cervical sampling	In house type-specifc primers and commercial type-specifc E6 primers for HPV16 and HPV18		77			77 (100)	All/HPV16/18	33.8		48.1	85.7		70.3		100.0
														Low grade/HPV16/18 (51)	12.8		28.2	18.7k		45.5		100.0
														High grade/HPV16/18 (38)	44.8		58.6	51.0k		76.5		100.0
														Cancer/HPV16/18 (12)	88.9		100	92.4k		88.9
Gupta et al30	India		Invasive cancer clinic patients		(41.7)		Prior to biopsy or cervical sampling	In house L1 consensus primers (any type = –)		30			28 (93.3)	All/any type	82.1		83.3d	100		100		100
			Healthy women (controls)		(42.1)					30				All/HPV16	67.9		70.0d	100		100		100
Song et al35	South Korea		Consecutively enrolled gynecological clinic patients		26–77 (45.2)		Two weeks after cervical sampling	HPV DNA chip (any type = 22 types)		100			30 (100)	All/any type	26.7		26.7	100		100		100
														All/HPV16	16.7		16.7	100		100		100
Payan et al32	France		Gynecological clinic patients. Gynecologist referred/consulting patients				First-void urine after cervical sampling	In house L1 consensus primers (any type = –)		333l			90 (90.0)	All/any type	52.2		70.0d	69.3k
														All/HPV16	34.4		38.0d	64.0k		65.9		95.7
														All/HPV18	3.3		5.0d	58.0k		40.0		98.8
														CIN/any type (48)	62.8		83.3d
														CIN/HPV16	37.2		35.4d
														CIN/HPV18	4.7		6.3d
														Cancer/any type (27)	70.8		89.7d
														Cancer/HPV16	50.0		62.1d
														Cancer/HPV18	4.2		6.9d
														C.Cervicitis/any type (26)	13.0		17.4d
														C.Cervicitis/HPV16	8.7		13.0d
														C.Cervicitis/HPV18	0		0
Bissett et al27	UK		Routine colposcopy clinic patients				Sampled at clinic	Modified GP primer protocol(HR-HPV = 13 types)		264			177 (100)	All/any type	37.3		45.0d	93.2k		91.2		96.3
Cuschieri et al18	Scotland		Recruited from a drop-in sexual health service clinic		16–25		Sampled at clinic	HPV INNO–LiPAe (any type = 27 types, type-specifc 27 types)		90			253 (95.8)	All/HR-HPV	70.4		80.6	57.9k		83.8		85.7
														All/HPV16/18	30.0		38.3	76.5k		75.3		98.1
														Normal/HR-HPV (20)	55.3		57.4			85.1		85.2
														Normal/HPV16/18	19.1		19.1			88.9		97.4
														Borderl/mild/HR-HPV (50)	70.8		82.5			83.8		90.5
														Borderl/mild/HPV16/18	26.7		35.0			76.2		100
														Mod/severe/HR-HPV (30)	79.2		91.7			84.8		83.3
														Mod/severe/HPV16/18	43.1		56.9			70.7		93.5
														All/any type	66.7		58.9	59.8k		90.6		67.6
														Type-specific HPV				70.8

Notes:aRefers to the assay used to detect overall HPV prevalence;

remaining samples were excluded for other reasons;

weighted prevalence;

based on “Total sample size” and not “Samples with human genomic DNA;”

HPV Genotyping Extra assay (Innogenetics);

urethral samples instead of urine;

paired urine and cervical samples from 343 females;

median value;

type-specific concordance calculated for HPV types for which five or more women had prevalent infection at least at one site;

incomplete for various reasons, including insufficient DNA;

kappa statistics;

only 177 urine samples were obtained.

Abbreviations: MY, MY09/MY11/(HMB01) primer system; GP, GP primer system; HCII, Hybrid capture II; E6, E6 primer system; Mod/severe, Moderate/Severe; Borderl, Borderline; HR, high risk; STD, sexually transmitted disease; LSIL, low-grade squamous intraepithelial lesions; HSIL, high-grade squamous intraepithelial lesions; ASCUS, atypical squamous cells of undetermined significance; CIN, cervical intraepithelial neoplasia; PCR, polymerase chain reaction; PAP, papanicolaou test; NA, not available; INNO-LIPA, (Innogenetics-line probe assay).

Figure 1

Human papillomavirus prevalence by age in urine samples from asymptomatic populations.

Abbreviation: HPV, human papillomavirus.

We identified 14 studies that measured HPV positivity in paired urine and cervical samples from symptomatic females;18,22,26–37 of these studies, nine reported the age range and nine the mean age of the study population. These studies included women with symptoms that led to various gynecological complaints and women diagnosed with invasive cervical cancer. Urine and cervical samples were collected at gynecological, colposcopy, genitourinary, sexually transmitted disease, and adolescent clinics. In general, HPV prevalence increased with the severity of cytological or pathological findings, and this was observed both in urine samples and cervical samples. All studies that reported age-specific HPV prevalence showed lower prevalence in urine samples than paired cervical samples, with the majority of the studies reporting a 10%–20% lower HPV prevalence, save the studies by Rymark et al33 and Cuschieri et al18 (Figure 2). With the exception of studies by Rymark et al33 and Jacobson et al,31 which covered narrow age ranges (16–21 years and 11–20 years, respectively), the studies in this review generally reported HPV prevalence in a broad age range. Populations presenting cytological or histological pathology generally had a higher HPV prevalence compared to those with normal cytology (Figures 1 and 2).

Figure 2

Human papillomavirus prevalence by age from paired urine and cervical samples from symptomatic populations (any HPV).

Notes: Dashed line represents urine samples, solid line represents cervical samples.

Abbreviation: HPV, human papillomavirus.

HPV concordance in paired urine and cervical samples

The studies showed a 75%–100% concordance for any HPV type in paired urine and cervical samples (or 41%–93% by kappa agreement). Type-specific concordance was reported in five studies, showing 100%, 90.5%, 71.0%, 70.8%, and 40.0% concordance. The latter estimates were calculated by including HPV-negative samples from either (not both) site, thereby reducing the type-specific concordance. Eight of the eleven studies published after 2000 also reported either type-specific concordance for HPV16 or HPV18, or concordance for the two types in combination. HPV16-specific concordance in the studies reviewed varied from 64%–100%.

HPV16-specific concordance or concordance for any HPV type by severity of cervical lesion was reported in three studies. Daponte et al28 showed an increase in HPV16/18-specific concordance with increasing severity. In contrast Alameda et al26 reported a higher concordance for any HPV type in low grade squamous intraepithelial lesion (LSIL) than in high grade squamous intraepithelial lesion (HSIL). Forslund et al29 showed neither an increase nor a decrease in concordance for any HPV type with increasing severity.

The only study that estimated sensitivity and specificity for HPV DNA detection in urine samples compared to cervical samples in a presumably asymptomatic, drop-in, sexual health service clinic population was published by Cuschieri et al18 who reported a sensitivity of 90.6% (95% confidence interval [CI] 79.3%–96.9%) and a specificity of 67.6% (95% CI 50.2%–82.0%). In the studies with symptomatic populations, the sensitivity varied from 52.9% to 100%. Specificity varied from 66.7% to 100%.

HPV positivity in males

We identified 14 male study populations from 13 publications that reported HPV positivity in urine samples and at least one other urogenital site (Table 2). Only the studies by Lazcano-Ponce et al38 and Cuschieri et al18 included males less than 18-years old. The 117 males aged 16–25 years in the Cuschieri et al18 study showed a 36.7% HPV prevalence in urine samples versus 29.1% in samples taken from the shaft of the penis. The study by Lazcano-Ponce et al38 included 120 healthy males aged 14–55 years in Mexico (43 males in the range 14–20 years) and reported a 6.9% and 42.7% HPV prevalence in urine samples and urethra samples, respectively. Similarly, HPV prevalence in the other studies listed in Table 2 was generally lower in urine samples than in other urogenital samples. For example, Weaver et al39 recruited 317 sexually active university students, aged 18–25 years, and measured HPV prevalence in urine samples as well as in samples from the glans, penile shaft, scrotum, and foreskin. Samples taken from the foreskin showed the highest prevalence (28.1%), while urine samples showed the lowest prevalence (5.8%).

Table 2

Studies with human papillomavirus (HPV) DNA detected in urine from males

Author	Country		Recruitment setting/patient characteristics	Age, years range (mean)	Urine sampling procedure	HPV types — assays (types detected)	Total sample size	Samples with human genomic DNA (%) (n)	HPV positivity (56)
Forslund et al29	Sweden		Presumably healthy conscripts randomly selected at a military campus	20–23 (21)	Not morning urine (clinic) Before urethra sampling	In house PCR (-)	143	Urine 96.5 (138)Urethra 96.5 (138)	5.88.7
Astori et al48	Italy		Recruited as partners of HPV positive women		First-void at bedtime (home), other samples morning	PCR with MY primers (≥36 types)	70	Urine 78.6 (55)Urethra 12.9 (9)Semen 100(70)	32.744.482.9
						Dot blot (−)		Urine 64.3 (45)Urethra 11.4(8)Semen 100(70)	26.737.551.4
Lazcano-ponce et al38	Mexico		Asymptomatic college students and industry workers recruited by a social worker	14–55(29.3)	First-void (home), without prior washing	PCR with GP primers (−)	I20a	Urine 30.2 (29)Urethra-coronal 100(96)	6.942.7
Rintala et al49	Finland		Healthy patients recalled for follow-up 6 months after vasectomy	33–9 (40.3)	Preejaculation (home), postejaculation (clinic)	PCR with MY primers (≥36 types) and GP primers (−)	27b	Preejac.urine 100(18)Postejac.urine 100 (18)Vas deferens 100 (27)Semen 100(18)	22.216.718.5 27.8
Fife et al50	USA		Males with no history of genital warts visiting STD clinic	18–50	First-void	PCR with HPV 6/11 specific primers (two types)	20	Urine 95.0 (19)Glans 70.0(l4)Penile shaft 90.0 (18)Scrotum 70.0(14)Inguinal area 60.0 (12)Perineum 45.0 (9)Perianal area 55.0 (11)	5.314.35.67.18.30.00.0
Weaver et al39	USA		Sexually active males recruited at university campus	18–25(20.5)	First-void (clinic)	PCR with MY primers (≥36 types)	317c	Urine 99.7 (313)Glans 97.5 (309)Penile shaft 98.1 (311)Scrotum 94.0 (298)Foreskind 98.3 (57)	5.816.524.817.828.1
Gupta et al30	India		Recruited as partners of women with cervical cancer	(46.4)	Before penile swab (clinic)	Any type = In house LI consensus	30	Urine 100(30)Genital area 100 (30)	66.766.7
			Recruited as partners of healthy women	(46.9)		primers (−)	30	Urine 100(30) Genital area 100 (30)	26.7 26.7
Giuliano et al20	USA		Healthy, sexually active, heterosexual males recruited at air force base and STD clinic	18–40(27.2)	First-void	PCR with MY primers (≥36 types)	463e	Urine 51.3 (116)Urethra 84.0 (278)Glans 95.9 (444)Penile shaft 97.0 (449)Scrotum 95.2 (441)Semen 98.0 (337)Perianal area 94.2 (436)Anal area 95.3 (386)	0.910.135.849.934.25.320.017.6
D′Hauwers et al51			Recruited as partners of HPV infected patients		First-void	PCR with MY primers (≥36 types)	30h	Urine 66.7 (20) Urethra-glans 100 (20)	0.0 60.0
Hernandez et al40	USA (Hawaii)		Healthy circumcised and uncircumcised recruitedat university campus	(29)	First-void (clinic)	PCR with MY primers (≥36 types)	379g=	Urine 57.0 (200)Glans 87.8 (308)Penile shaft 95.1 (334)Scrotum 88.3 (310)Semen 56.1 (197)Foreskind 78.8 (63)	10.032.552.439.76.144.4
Shigehara et al52	Japan	Males with urethritis visiting STD clinic, outpatient clinics and hospitals		19–62(35.2)	(clinic)	PCR with GP primers (−)	142	Urine 64.8 (92)Urethra 93.0 (132)Glans 89.4 (127)	24.019.731.5
Bissett et al27	UK	Uncircumcised males with multiple sexual partners or a diagnosis of genital warts in the last 6 months visiting a genitourinary medicine clinic			(clinic)	Modified GP primer protocol (13 types)	88	Urine 98.9 (87)Genital area 98.9 (87)(Glans, shaft, scrotum, foreskin)	16.149.4
Cuschieri et al18	Scotland	Recruited from a drop-in sexual health service clinic		16–25	(clinic)	HPV INNO-LiPAh (27 types)	117	Urine Penile shaft	36.829.1

Notes:aAnalyses based on sexually active males only (n = 96);

b18 samples from urine and semen;

cthree urine samples were not obtained;

duncircumcised males only;

e226 urine samples were obtained;

f20 samples from the urethro glandular;

gCircumcised (n = 299) and uncircumcised males (n = 80), 351 males after excluding for HIV infection;

hHPV Genotyping Extra assay (Innogenetics).

Abbreviations: n, adequate samples; MY, MY09/MYIl/(HMB0l) primer system; GP, GP primer system; STD, sexually transmitted disease; PCR, polymerase chain reaction; PAP, Papanicolaou test; INNO-LIPA, (Innogenetics-line probe assay)

The percentage of urine samples in which human genomic DNA could be detected varied substantially between the studies. While Weaver et al39 detected human genomic DNA in 99.7% of urine samples and 94.0%–98.3% of samples from other sites, Giuliano et al only detected human genomic DNA in 51.3% of urine samples and 84.0%–98.0% of samples from other sites, with semen samples having the highest human genomic DNA detection rate. In the study by Hernandez et al,40 semen samples and urine samples had the lowest human genomic DNA detection rate, with 56.1% and 57.0%, respectively, compared to 78.8%–95.1% from other urogenital sites.

Technical issues affecting human genomic DNA and HPV DNA detection

To illustrate some of the technical variability in these studies, we have listed the urine sampling procedure and the DNA detection method used (Tables 1 and 2). The most common urine sampling procedure in both female and male populations was first-void urine in contrast to mid-stream urine, which Vorsters et al17 suggested would be preferable if the goal were to analyze a maximum number of exfoliated cells. The order of urine and cervical sampling may also affect the HPV DNA detection rate in urine, and some studies have suggested that it is preferable to collect the urine sample first (reviewed in Sehgal et al).21 In the female populations listed in Table 1, urine sampling was not always carried out prior to cervical sampling and was sometimes done after washing the genitals. For HPV DNA detection, variants of the MY09/MY11 primer were most commonly used, but other primers, such as general primer GP5+/6+, in-house primers, E6-primers, hybrid capture II, and DNA chip assays were also used. In summary, the technical variability may contribute substantially to HPV DNA detection rates.

Discussion

According to the World Health Organization (WHO), 33 countries have implemented HPV vaccination as part of their national immunization program.41 Generally, vaccination is provided to girls, and it is therefore recommended to monitor the impact of vaccination on HPV prevalence among female adolescents.15 In August 2012, we identified four publications that reported HPV prevalence in urine samples from asymptomatic female adolescents. HPV prevalence has been strongly associated with age, being nearly nonexistent in preadolescents, gradually increasing with sexual activity among adolescents, and generally peaking around 25 years of age.42 However, regional differences in HPV prevalence do exist.43 Therefore, the first step when monitoring HPV prevalence is to establish the baseline HPV prevalence in the relevant age groups. To date, only Hussain et al and O’Leary et al reported baseline HPV prevalence based on urine samples from a large unvaccinated adolescent population.24,25 The Hussain et al25 study from India used self-collected urine of the cervix and that care should be taken when samples from healthy children attending public school and achieved a 57.3% participation rate. O’Leary et al24 analyzed urine samples from 11–18-year-old school and college males (1121) and females (1341) in Scotland 4 months before vaccination was introduced in the national immunization schedule in 2008. A limitation of the study was that the estimated response rate for providing a urine sample was as low as 14%. While the low response rate can introduce bias and lead to erroneous estimates of the overall HPV prevalence, it was not directly related to the sampling method and probably refects a general challenge to achieve high response rates in this age group. This, in turn, could partially explain why only few studies measuring HPV prevalence in urine samples from female adolescents in the general population have been performed and published.

The five studies that reported HPV prevalence by lesion severity showed a similar association for paired urine and cervical samples, with higher HPV prevalence in the most severe lesions. There were major variations in HPV prevalence in urine samples across the studies. This is to some degree related to regional differences in HPV prevalence,43 the age distribution of the different study populations,43 and the setting in which the women were recruited. There were also differences in sampling procedures and HPV detection methods, including the number of types detected by a given assay. It is therefore not possible, as Vorsters et al17 pointed out, to perform a meta-analysis on the present urine-based HPV prevalence studies.

Detection of human genomic DNA is commonly used to control for the adequacy of samples for HPV detection. Studies including female populations showed a high detection rate of human genomic DNA in urine samples (83%–100%), while male populations showed a larger range of detection rates (30%–100%). In an HPV monitoring setting, a low human genomic DNA detection rate would lead to reduced coverage and create a concern of bias in HPV estimates. In general, studies on female populations in this review indicated that high detection rates of human genomic DNA are feasible.

In cervical screening the main focus is to detect HPV or cervical abnormalities at the individual level, while population-based HPV prevalence is used more in a monitoring or epidemiological setting. Therefore, although prevalence in urine samples was lower than in cervical samples in the studies included in this review, monitoring by regular urine measurements over time may still be a useful way of identifying shifts in HPV prevalence due to imparted immunity against vaccine HPV types. However, the differences in HPV concordance of paired urine and cervical samples illustrates that HPV positivity in urine should be interpreted independently of the cervix and that care should be taken when inferring that a similar change is taking place in the cervix. On the other hand HPV detection in urine samples could be considered an independent measurement of the impact of HPV vaccination but it would have only limited public health interest. Furthermore, we observed that HPV negativity in the cervix commonly predicted an HPV-negative result in the urine as well, while HPV positivity in the cervix less commonly predicted HPV positivity in the urine. Although Daponte et al showed an increased concordance with increased lesion severity for any HPV type, other studies like Alameda et al,26 Rymark et al,33 and Gupta et al30 showed a relatively high concordance, even in populations where HPV prevalence is low. The variability of HPV16/18-specific concordance, the types included in both of the available HPV vaccines, further exemplifies the uncertainty of using urine samples to estimate future changes in the incidence of cervical lesions.

The most comprehensive monitoring of changes in HPV prevalence would be carried out by establishing baseline HPV prevalence before measuring any impact of vaccination as well as regular measurements of HPV prevalence in both vaccinated and unvaccinated females and males. The age group (or groups) and sample size to include in HPV monitoring should be carefully selected to assure there is enough statistical power to identify changes in overall HPV prevalence as well as HPV type-specific changes. Models suggest that there will be a significant reduction in the prevalence of vaccine HPV types in males in the future because after vaccination, fewer girls will transmit HPV to their male partners.44 Monitoring HPV prevalence in males could therefore be a near-term end point that could also help to estimate the effect of herd immunity. However, monitoring HPV prevalence in males presents several challenges. The differences in HPV prevalence across different urogenital sites illustrates that no single site repeatedly shows the highest HPV DNA detection rate and that urine in particular has a relatively low HPV DNA detection rate compared to other sites. In addition, male urine generally has a lower detection rate for human genomic DNA than samples from other urogenital sites. With lower detection rates for human genomic DNA, a larger sample size would be needed to detect changes with the same power as other urogenital sites. Based on these aspects, other anatomical sites seem more favorable for males.

Monitoring changes in HPV prevalence requires regular prevalence measurements over many years. A protocol with sufficient detail on technical and practical issues that influence HPV detection is therefore necessary to ensure comparability between these measurements. This includes, among other issues, urine sampling procedure, handling of samples, extraction of DNA, and assay used for HPV genotyping.17 In addition it might be useful to store an extra aliquot of extracted DNA from each regular measurement to be able to perform HPV genotyping on all DNA collected from urine samples over many years. This would also allow for using any novel genotyping technology that may have developed during the monitoring period. Information on more aspects of HPV monitoring can also be found in the Human Papillomavirus Laboratory Manual issued in 2009 by the WHO HPV Laboratory Network (WHO HPV LabNet).45 This manual covers guidance on specimen collection and handling for HPV testing, with the aim to assist in establishing the laboratory support required for implementation and monitoring of HPV vaccination programs. Several of the WHO HPV LabNet members are actively undertaking studies of HPV detection in urine, and a leading role for the WHO HPV LabNet in further standardizing and optimizing the technology for HPV detection in urine seems appropriate.18,45,46

This is the first review that focuses solely on the use of urine to monitor changes in HPV prevalence in an asymptomatic population. The major shortcoming of this review is that, to date, there are few studies on the topic. We have therefore included studies from symptomatic populations and older populations that used urine for purposes other than monitoring, although these are not comparable to asymptomatic adolescents in all aspects. In addition, the studies highlighted in the present review as well as in the reviews of Vorsters et al17 and Seghal et al,21 showed that the large variability in sampling and genotyping methodology make direct comparisons of data, like concordance, inaccurate.17,21

Assuming a future reduction in overall HPV prevalence and vaccine HPV type-specific prevalence and using urine testing as a monitoring method, care should be taken when interpreting the data. Indeed the data may not necessarily mimic the true HPV distribution in the cervix nor estimate the expected reductions in cervical cancer and high-grade lesions, as indicated by variable vaccine HPV type-specific (HPV16/18) concordance between paired urine and cervical samples. There is great scientific and political interest in monitoring the early effects of HPV vaccination in the general population. However, monitoring HPV prevalence as an early measurement of vaccine impact is only possible in a few countries as substantial financial and human resources are needed as well as a 5–10-year commitment in order to demonstrate results.16

Conclusion

Urine is an adequate alternative biospecimen for monitoring HPV prevalence in female adolescents to determine the early effect of HPV vaccination on a population level. Strategies for recruitment should be optimized to avoid low response rates, sampling and HPV detection protocols should be detailed and standardized to ensure comparability, and importantly, care should be taken when extrapolating findings to the cervix. In males, urine samples do not seem to be optimal for monitoring HPV prevalence due to a low human genomic DNA content compared to other urogenital sites. Although urine sampling has some advantages and is the only relevant option for sampling the general population in the youngest age groups, it also has several disadvantages, most importantly the fact that HPV prevalence in urine is only a distant measure of the main end point of vaccine impact, cervical cancer. In each situation the costs and benefits of HPV DNA detection in urine, compared to alternative monitoring options, should be carefully considered.16,47