Enterovirus serotyping includes identification of the following: Coxsackie virus serotypes A9, A24, and B1-6; Echovirus serotypes 4, 6, 9, 11, and 30; Enterovirus serotypes 70 and 71; and Polioviruses 1, 2, and 3.

This test is approved for New York patient testing.

This assay is a selective and differential culture for isolation of E. coli phenotypes that lack the ability to ferment sorbitol, a key characteristic of E. coli O157:H7 serotype. Most other serotypes of E. coli ferment sorbitol. Sorbitol negative isolates identified as E. coli will have O157:H7 serotyping performed at an additional charge. This test does not detect the disease associated Shiga- toxin nor does this test detect E. coli serotypes other than O157:H7 that may produce Shiga-toxin. Please request E. coli, Enterohemorrhagic (EHEC), Shiga-like toxin detection, EIA (Focus Unit Code 52068) if Shiga-toxin testing is required. For culture of E. coli other than O157:H7, please refer to Focus test “Bacterial Culture, Aerobic, Special” (Focus Unit Code 51250) and request E. coli. For serotyping E. coli isolates for O157:H7, refer to Focus test “E. coli O157:H7 Serotyping” (Focus Unit Code 52065).

This test is not approved for New York patient testing.

This assay detects all known enteroviruses and parechoviruses. These viruses are a common cause of nonspecific febrile illness and meningitis in children and adults. Parechoviruses are genetically distinct from enteroviruses and will not be detected in a pan-enterovirus RT-PCR assay.

This test is not approved for New York patient testing.

This assay tests for two antibody specificities:
1. Antibody to intercellular substance of the epidermis. This antibody strongly suggests the diagnosis of pemphigus (all forms), although it may be rarely present in burn patients and trichophyton infections. The rise and fall of the titer may be indicative of relapse and remission of the disease respectively.
2. Antibody to the dermal-epidermal basement membrane. This antibody is highly specific for bullous pemphigoid and is present in 80% of these patients.

This test is approved for New York patient testing.

This unit code has been inactivated.

Please see unit code 52069.

The detection of Epstein-Barr virus (EBV) DNA is based upon the real-time amplification and detection of specific EBV genomic DNA sequences by PCR from total DNA extracted from the specimen.

This test is approved for New York patient testing.

Quantitation of EBV DNA is based upon the real-time PCR amplification and detection of EBV genomic DNA. The quantitative range of this assay is from 200 to 2,000,000 EBV DNA copies/mL.

This test is approved for New York patient testing.

E. coli O157:H7 has emerged as an enteric pathogen of public health importance causing outbreaks of diarrhea, hemorrhagic colitis, and hemolytic uremic syndrome. Although multiple serotypes have been reported to cause disease, the O157:H7 serotype is the most common single strain isolated. Not all O157 strains have the H7 flagellar antigen. This test is performed to confirm identification of the O157:H7 serotype of E. coli. To confirm or detect Shiga-toxin activity of an E. coli O157:H7 isolate, the Shiga-toxin detection EIA is recommended. Please request E. coli, Enterohemorrhagic (EHEC), Shiga-Like Toxin EIA (Focus Unit Code 52068) if toxin detection is required.

This test is approved for New York patient testing.

If EBV DNA is detected in the qualitative assay, the specimen will reflex to EBV Quantitative PCR (Focus Unit Code 48453) for an additional charge. The quantitative range if reflexed is 200 - 2,000,000 EBV DNA copies/mL.

This test is approved for New York patient testing.

Antibody to the EBV nuclear antigen (EBNA) appears no earlier than 3-4 weeks post-onset of primary EBV infection, with many patients requiring several months to produce detectable antibody. Titers >=1:160 generally rule out a diagnosis of primary EBV infection.

This test is approved for New York patient testing.

Enterohemorrhagic E. coli (EHEC) have been isolated from patients with hemorrhagic colitis and hemolytic-uremic syndrome, and can produce bloody diarrhea secondary to toxin damage of vascular endothelial cells. A large portion of EHEC isolates belong to the serotype 0157:H7, although at least 50 other EHEC serotypes have been reported. All EHEC strains produce potent cytotoxins called Shiga-like toxins or verotoxins, which are biochemically similar to the Shiga toxin produced by strains of Shigella dysenteriae serotype 1. This very sensitive assay detects the presence of Shiga-like Toxins 1 and 2 directly in stool specimens or culture systems.

This test is approved for New York patient testing.

Detection of intrathecally-produced organism-specific antibodies in CSF indicates central nervous system infection. However, serum levels of organism-specific antibodies, blood-brain barrier integrity, and possible CSF contamination by blood should be considered when assessing CSF results.

This test is approved for New York patient testing.

EBNA IgM is often detected in recent or current Epstein Barr Virus (EBV) infection. However, EBNA IgM is also found in 2-12% of healthy adults, depending on age and geographic location.

This test is approved for New York patient testing.

Both IgG and IgM antibody levels are titered. A four-fold increase in VCA-lgG or a VCA-lgM titer >=1:20 is indicative of current infection.

This test is approved for New York patient testing.

Detection of intrathecally-produced organism-specific antibodies in CSF indicates central nervous system infection. However, serum levels of organism-specific antibodies, blood-brain barrier integrity, and possible CSF contamination by blood should be considered when assessing CSF results.

This test is approved for New York patient testing.

EBV VCA IgG and IgM are stimulated in virtually all primary EBV infections. VCA-IgM appears immediately after onset of symptoms and usually disappears within 2-3 months. VCA-IgG appears immediately after onset of symptoms and persists indefinitely, falling gradually with time unless restimulated as in reactivated infection and chronic disease.

This test is approved for New York patient testing.

This unit code has been inactivated.

Please see unit code 52068.

IgG titers >=1:16 suggest exposure, while the presence of IgM indicates recent infection. Human infections are seasonal, from mid- to late-summer, occurring from New England to Texas. Minimal crossreactivity with other Group A arboviruses, i.e., Western Equine Encephalitis virus, occurs.

This test is approved for New York patient testing.

Detection of intrathecally-produced organism-specific antibodies in CSF indicates central nervous system infection. However, serum levels of organism-specific antibodies, blood-brain barrier integrity, and possible CSF contamination by blood should be considered when assessing CSF results.

This test is available for New York patient testing.

Detection of intrathecally-produced organism-specific antibodies in CSF indicates central nervous system infection. However, serum levels of organism-specific antibodies, blood-brain barrier integrity, and possible CSF contamination by blood should be considered when assessing CSF results.

This test is approved for New York patient testing.

IgG titers >=1:16 suggest exposure, while the presence of IgM indicates recent infection. Human infections are seasonal, from mid- to late-summer, occurring from New England to Texas. Minimal crossreactivity with other Group A arboviruses, i.e., Western Equine Encephalitis virus, occurs.

This test is approved for New York patient testing.

VCA-IgG appears immediately after onset of symptoms and persists indefinitely. VCA-IgA titers between 1:10 and 1:80 suggest past infection, whereas titers greater than 1:80 suggest chronic infection.

This test is approved for New York patient testing.

EBV VCA IgG and IgM are stimulated in virtually all primary EBV infections. VCA-IgM appears immediately after onset of symptoms and usually disappears within 2-3 months. VCA-IgG appears immediately after onset of symptoms and persists indefinitely, falling gradually with time unless restimulated as in reactivated infection and chronic disease.

This test is approved for New York patient testing.

Detection of intrathecally-produced organism-specific antibodies in CSF indicates central nervous system infection. However, serum levels of organism-specific antibodies, blood-brain barrier integrity, and possible CSF contamination by blood should be considered when assessing CSF results.

This test is available for New York patient testing.

IgG titers >=1:16 suggest exposure, while the presence of IgM indicates recent infection. Human infections are seasonal, from mid- to late-summer, occurring from New England to Texas. Minimal crossreactivity with other Group A arboviruses, i.e., Western Equine Encephalitis virus, occurs.

This test is approved for New York patient testing.

Detection of intrathecally-produced organism-specific antibodies in CSF indicates central nervous system infection. However, serum levels of organism-specific antibodies, blood-brain barrier integrity, and possible CSF contamination by blood should be considered when assessing CSF results.

This test is approved for New York patient testing.

A transient elevation in titer is seen in 85% of acute EBV infections. Although titer increases may appear at a later date due to an asymptomatic viral reactivation, elevated levels (>=1:640) may also be related to chronic or reactivated EBV. Titers are also elevated in Burkitt's lymphoma and nasopharyngeal carcinoma.

This test is approved for New York patient testing.

Detection of intrathecally-produced organism-specific antibodies in CSF indicates central nervous system infection. However, serum levels of organism-specific antibodies, blood-brain barrier integrity, and possible CSF contamination by blood should be considered when assessing CSF results.

This test is available for New York patient testing.

Detection of serum antibodies to Echinococcus plays an important role in the diagnosis of hydatid disease, since infected individuals do not exhibit fecal shedding of Echinococcus eggs. Increasing antibody values between acute and convalescent specimens is considered evidence of recent or current infection. The frequency of a positive result for serum antibodies to Echinococcus is higher in patients with active cysts in the liver than in patients with hydatid cysts in the lung or calcified cysts. Serologic crossreactivity between Echinococcus and Cysticercus may occur.

This test is approved for New York patient testing.

Detection of intrathecally-produced organism-specific antibodies in CSF indicates central nervous system infection. However, serum levels of organism-specific antibodies, blood-brain barrier integrity, and possible CSF contamination by blood should be considered when assessing CSF results.

This test is approved for New York patient testing.

This unit code has been inactivated.

Please see unit code 2420.

The current Echovirus panel includes serotypes 4, 7, 9, 11 and 30. The Echovirus serotypes used in this panel will vary depending upon current epidemiological data available from in-house isolations and CDC reports. Generally, the serotypes used are those most commonly associated with viral meningitis. Although there is crossreactivity among the enteroviruses, most healthy people do not have detectable CF titers (>1:8). Therefore, detectable titers, especially those >=1:32, should be considered a positive identification. Confirmation is made by demonstration of a four-fold change in titers between acute and convalescent sera. See Unit Code 4403 for parallel testing.

This test is approved for New York patient testing.

The primary panel is used for the diagnosis of acute primary EBV infection. It includes Epstein-Barr nuclear antigen (EBNA) antibody at a dilution of 1:10, as well as IgG and IgM antibodies to the viral capsid antigen (VCA) at dilutions of 1:10 and 1:20 respectively.

	Acute Infection	Primary Infection	Past Infection
Months	1	2	3
VCA-IgG	>=1:10	>=1:10	>=1:10
VCA-IgM	>=1:20	<1:20	<1:20
EBNA ACIF	<1:10	<1:10	>=1:10

EBV VCA IgG and IgM are stimulated in virtually all primary EBV infections. VCA-IgM appears immediately after onset of symptoms and usually disappears within 2-3 months. VCA-IgG appears immediately after onset of symptoms and persists indefinitely, falling gradually with time unless restimulated as in reactivated infection and chronic disease. EBNA antibody can be detected 2-6 months after acute illness, and usually persists for life.

Detection of intrathecally-produced organism-specific antibodies in CSF indicates central nervous system infection. However, serum levels of organism-specific antibodies, blood-brain barrier integrity, and possible CSF contamination by blood should be considered when assessing CSF results.

This test is approved for New York patient testing.

VCAIgA titers above the reference range are suggestive of chronic or reactivated EBV infection. Detectable titers within the reference range are due to past infection.

This test is approved for New York patient testing.

See individual assay for description.

Panel Includes:

• Epstein-Barr Nuclear Antigen (EBNA) Antibody, ACIF
• Epstein-Barr Virus (EBV) VCA and IgM Antibody Panel IFA

Detection of intrathecally-produced organism-specific antibodies in CSF indicates central nervous system infection. However, serum levels of organism-specific antibodies, blood-brain barrier integrity, and possible CSF contamination by blood should be considered when assessing CSF results.

This test is approved for New York patient testing.

This unit code has been inactivated.

Please see unit code 40435.

• Enterovirus RNA, Qualitative Real-Time PCR

This panel detects antibody responses to EBV which may suggest chronic infection. Specimens with titers above the reference ranges (see below) are suggestive of chronic or reactivated EBV infection. Titers within the reference ranges are due to past infection.

		Reference Range
	VCA IgG-IFA:	1:10-1:2560
	VCA IgA-IFA:	1:10-1:80
	EA (R + D) IgG-IFA:	1:10-1:320

Many cases of chronic EBV disease display elevated EBV titers. However, it is difficult to diagnose serologically due to the variations of antibody responses possible. The Viral Capsid Antigen (VCA) IgG appears immediately after primary infection and persists indefinitely, falling gradually with time unless restimulated as in reactivated infection or chronic disease. The VCA-IgA is considered an acute phase antibody and its presence at elevated levels may be related to chronic or reactivated EBV infection. Titers to EA are generally detectable at onset of acute primary disease and begin to fall in 3-6 months. However, many cases of chronic EBV disease display elevated EA titers.

• Ehrlichia chaffeensis Antibodies (IgG, IgM)
• Ehrlichia chaffeensis DNA Real-Time PCR

Specimens collected just before or within 15 minutes of the next dose represent the TROUGH levels. Specimens obtained within 15-30 minutes after the end of I.V. infusion or 45-60 minutes after an IM injection or 90 minutes after oral intake represent the PEAK level.

This test is available for New York patient testing.

See individual assay for description.

Panel Includes:

• Epstein-Barr Nuclear Antigen (EBNA) Antibody, ACIF
• Epstein-Barr Viral Capsid Antigen IgG and IgM Antibody, IFA
• Epstein-Barr Virus Early Antigen (R+D) IgG, IFA

See individual assay for description.

Panel Includes:

• Epstein-Barr Nuclear Antigen (EBNA) Antibody, ACIF
• Epstein-Barr Viral Capsid Antigen IgG and IgM Antibody, IFA
• Epstein-Barr Virus Early Antigen (R+D) IgG, IFA

Ehrlichia chaffeensis DNA detection is based on real-time PCR, a highly sensitive method to detect the presence of microbial nucleic acid in clinical specimens.

This test is not approved for New York patient testing.

See individual assay for description.

Panel Includes:

• Epstein-Barr Nuclear Antigen (EBNA) Antibody, ACIF
• Epstein-Barr Viral Capsid Antigen (VCA) IgG Antibody, IFA
• Epstein-Barr Virus Early Antigen (R+D) IgG, IFA

Ehrlichia chaffeenis has been identified as the causative agent of Human Monocytic Ehrlichiosis (HME). Infected individuals produce specific antibodies to E. chaffeensis that can be detected by an immunofluorescent antibody (IFA) test. Single IgG IFA titers of 1:64 or greater indicate exposure to E. chaffeensis. A four-fold rise in IgG titers between acute and convalescent samples and/or the presence of IgM antibody against E. chaffeensis suggest recent or current infection.

†This test was developed and its performance characteristics determined by Focus Diagnostics. It has not been cleared or approved by the U.S. Food and Drug Administration. The FDA has determined that such clearance or approval is not necessary. Performance characteristics refer to the analytical performance of the test.

This test is approved for New York patient testing.

• Parvovirus (B19) Antibody Panel, ELISA and DNA, PCR
• Parvovirus (B19) Antibody Panel, RIFA and DNA, PCR
• Parvovirus (B19) IgM Antibody, RIFA
• Parvovirus B19 DNA, Qualitative Real-Time PCR
• Parvovirus B19 DNA, Qualitative To Quantitative Real-Time PCR Reflex
• Parvovirus B19 DNA, Quantitative Real-Time PCR

Genes associated with beta-lactamase-mediated ampicillin resistance in E. coli and Klebsiella pneumoniae can undergo simple point mutations that result in the production of beta-lactamases that are capable of hydrolyzing broad spectrum beta-lactam antibiotics such as ceftazidime, cefotaxime, ceftriaxone, and aztreonam. These plasmid-mediated extended spectrum beta-lactamases (ESBLs) are generally inhibited by beta-lactamase inhibitors, e.g., clavulanic acid, sulbactam, and tazobactam, and are currently not active against cefamycins and carbapenems. ESBLs have been most commonly documented in E. coli and Klebsiella pneumoniae strains, but reports have indicated their spread to other species of the family Enterobacteriaceae.

Detection of ESBL expression has proven to be difficult for many laboratories, and the CLSI (formerly NCCLS) has recommended specific criteria for ESBL confirmation using the preferred substrates ceftazidime and cefotaxime. These two antimicrobial agents, alone and in combination with clavulanic acid, are tested by standard disk diffusion methods, and a >=5 mm increase in zone diameter for either antimicrobial agent tested in combination with clavulanic acid versus its zone when tested alone is confirmatory for the presence of ESBL. This method has been recommended for use only with E. coli and Klebsiella spp. and may not be appropriate for other enteric gram-negative bacilli. If ESBL production is confirmed, the bacterial isolate should be considered as resistant to all penicillins, cephalosporins, and aztreonam.

This test is approved for New York patient testing.

One of the causes of granulocytic ehrlichiosis in dogs, E. ewingii is now known to cause human infection as well. Disease is transmitted by the lone star tick and less commonly by other tick species. As with E. chaffeensis, human disease is seen predominantly in the southeastern and south-central parts of the U.S. Clinical symptoms include fever, headache, and thrombocytopenia, with or without leucopenia.

This test is not approved for New York patient testing.

• Anaplasma phagocytophilum and Ehrlichia chaffeensis Antibody Panel

• RNP and Sm Antibodies IgG, MAID
• SS-A and SS-B IgG Antibodies, MAID

• Extractable Nuclear Antigen (ENA) Antibody Panel, MAID

See individual assay for description.

Panel Includes:

• RNP and Sm Antibodies IgG, MAID
• Scl-70 Antibody IgG, MAID
• SS-A and SS-B IgG Antibodies, MAID

• Meningoencephalitis (Encephalitis) Panel (CSF)
• Meningoencephalitis (Encephalitis) Panel (Serum)
• Meningoencephalitis Comprehensive Panel (CSF)
• Meningoencephalitis Comprehensive Panel (Serum)

See individual assay for description.

Panel Includes:

• Herpes Simplex Virus (HSV) 1/2 IgM and Type-Specific IgG (HerpeSelect®), ELISA
• Lymphocytic Choriomeningitis (LCM) IgG and IgM Antibody, IFA
• Measles (Rubeola) IgG and IgM Antibody Panel, IFA
• Mumps IgG and IgM Antibody, IFA and
• Varicella-Zoster Virus Antibody Total and IgM, ACIF/IFA

See individual assay for description.

Panel Includes:

• Herpes Simplex Virus (HSV) 1/2 Antibody, ACIF
• Herpes Simplex Virus (HSV) 1/2 IgM Panel, IFA
• Lymphocytic Choriomeningitis (LCM) IgG and IgM Antibody, IFA
• Measles (Rubeola) IgG and IgM Antibody Panel, IFA
• Mumps IgG and IgM Antibody, IFA
• Varicella-Zoster Virus Antibody Total and IgM, ACIF/IFA

IgA endomysial antibody is present in approximately 70% of dermatitis herpetiformis (DH) patients and nearly 100% of celiac disease patients not on gluten-free diets. Decreasing antibody titers correlate with adherence to a gluten-free diet.

This test is approved for New York patient testing.

 Serologic Tests for Celiac Disease

• Limulus Amebocyte Lysate (LAL) Assay, Quantitative

The detection of Entamoeba histolytica antigen by immunoassay is a highly sensitive and specific test. It is extremely useful in cases of amebiasis where ova and parasite examinations are inconclusive. This assay will detect only the antigen of the pathogenic E. histolytica; it will not detect the non-pathogenic E. dispar.

This test is approved for New York patient testing.

Serologic studies may be helpful in the diagnosis of invasive intestinal and extra-intestinal amebiasis. Asymptomatic cyst passers usually have negative serologic tests. Eighty-five percent of patients with biopsy proven invasive intestinal amebiasis are antibody positive whereas 95-100% of patients with extra-intestinal amebiasis are positive. Values may remain elevated 6 to 18 months following invasive disease.

This test is approved for New York patient testing.

This unit code has been inactivated.

Please see unit code 40105.

Reverse transcriptase-PCR (RT-PCR) is a highly sensitive method used to detect Enterovirus (EV) RNA from various clinical specimens. This assay targets a conserved region of the EV genome which allows detection of nearly the entire spectrum of human Enteroviruses, including the Coxsackieviruses, Polioviruses and the Echoviruses. It does not differentiate among the EV serotypes.

This test is not approved for New York patient testing.

See individual assay for description.

Panel Includes:

• Coxsackie Type B Antibody Panel, CF
• Echovirus Antibody Panel, CF
• Poliovirus (Types 1-3) Antibody, CF

See individual assay for description.

Panel Includes:

• Coxsackie Type B Antibody Panel, CF
• Echovirus Antibody Panel, CF
• Poliovirus (Types 1-3) Antibody, CF

See individual assay for description.

Panel Includes:

• Coxsackie Type A Antibody Panel, CF
• Coxsackie Type B Antibody Panel, CF
• Echovirus Antibody Panel, CF
• Poliovirus (Types 1-3) Antibody, CF

See individual assay for description.

Panel Includes:

• Coxsackie Type A Antibody Panel, CF
• Coxsackie Type B Antibody Panel, CF
• Echovirus Antibody Panel, CF
• Poliovirus (Types 1-3) Antibody, CF

The Enterovirus Culture utilizes two genetically transformed cell lines for enhanced viral recovery and more rapid viral detection when compared to conventional cell line methods. If isolated, Enterovirus will be identified using a pan-enterovirus fluorescent antibody stain method.

This test is approved for New York patient testing.

This unit code has been inactivated.

Please see unit code 88250.