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Genetic variation of SARS coronavirus in Beijing hospital.


To characterize genetic variation of severe acute respiratory syndrome-associated coronavirus coronavirus /co·ro·na·vi·rus/ (ko-ro´nah-vi?rus) any virus belonging to the family Coronaviridae.
Coronavirus /Co·ro·na·vi·rus/ (ko-ro´nah-vi?rus 
 (SARS-CoV) transmitted in the Beijing area during the epidemic outbreak of 2003, we sequenced 29 full-length S genes of SARS-CoV from 20 hospitalized SARS patients on our unit, the Beijing 302 Hospital. Viral RNA RNA: see nucleic acid.
RNA
 in full ribonucleic acid

One of the two main types of nucleic acid (the other being DNA), which functions in cellular protein synthesis in all living cells and replaces DNA as the carrier of genetic
 templates for the S-gene amplification were directly extracted from raw clinical samples, including plasma, throat swab, sputum sputum /spu·tum/ (spu´tum) [L.] expectoration; matter ejected from the trachea, bronchi, and lungs through the mouth.

sputum cruen´tum  bloody sputum.
, and stool, during the course of the epidemic in the Beijing area. We used a TA-cloning assay with direct analysis of nested reverse transcription--polymerase chain reaction products in sequence. One hundred thirteen sequence variations with nine recurrent variant sites were identified in analyzed S-gene sequences compared with the BJ01 strain of SARS-CoV. Among them, eight variant sites were, we think, the first documented. Our findings demonstrate the coexistence of S-gene sequences with and without substitutions (compared to BJ01) in samples analyzed from some patients.

**********

A novel severe acute respiratory syndrome--associated coronavirus (SARS-CoV) has been implicated im·pli·cate  
tr.v. im·pli·cat·ed, im·pli·cat·ing, im·pli·cates
1. To involve or connect intimately or incriminatingly: evidence that implicates others in the plot.

2.
 as the causative agent of a worldwide outbreak of SARS during the first 6 months of 2003 (1-3). From March 4 to June 18, Beijing had 2,521 cases and 192 deaths from SARS (4). Because of the poor fidelity of RNA-dependent RNA polymerase RNA polymerase
n.
A polymerase that catalyzes the synthesis of RNA from a DNA or RNA template.
, genetic variation typically forms a heterogeneous virus pool in RNA virus RNA virus
n.
Any of a group of viruses whose nucleic acid core is composed of RNA, including the picornaviruses, retroviruses, and paramyxoviruses.
 populations, including coronaviruses such as mouse hepatitis virus Mouse hepatitis virus is a virus of the family Coronaviridae, genus coronavirus. References
  • University of Illinois entry (PDF)
 (MHV MHV

mouse hepatitis virus.
) (5,6). This feature makes viruses highly adaptable and contributes to difficulties in preventing and controlling viral disease. SARS-CoV, a single-stranded RNA virus, has been reported with relatively less variability in analyses of a limited number of viral isolate collections (7-10). Furthermore, no SARS-CoV quasispecies have been documented, as they have been in many other RNA viruses RNA viruses,
n See viruses.
, including hepatitis C virus
This page is for the virus. For the disease, see Hepatitis C.
The Hepatitis C virus (HCV) is a small (50 nm in size), enveloped, single-stranded, positive sense RNA virus in the family Flaviviridae.
 (HCV HCV
abbr.
hepatitis C virus


HCV 1 Hepatitis C virus, see there 2. Human coronavirus. See Coronavirus.
) (11), H1V (12), and MHV (6).

During the SARS outbreak in Beijing, 132 SARS patients were hospitalized and treated on our unit at Beijing Hospital, including the first cluster of case-patients in the area (13). To characterize genetic variation among SARS-CoV transmitted in the Beijing area, we sequenced 29 full-length S genes of SARS-CoV from 20 hospitalized SARS patients, since S glycoprotein glycoprotein (glī'kōprō`tēn), organic compound composed of both a protein and a carbohydrate joined together in covalent chemical linkage.  plays a key role in virus-host interaction and is predicted to be the main target of immune response immune response
n.
An integrated bodily response to an antigen, especially one mediated by lymphocytes and involving recognition of antigens by specific antibodies or previously sensitized lymphocytes.
 (14). Samples that were analyzed represented the timespan of the epidemic. To exclude culture-derived artifacts artifacts

see specimen artifacts.
 and estimate mutational heterogeneity, viral RNA was directly extracted from raw clinical samples, and a TA-cloning assay was used with direct analysis of reverse transcriptase-polymemse chain reaction (RT-PCR RT-PCR

reverse transcriptase-polymerase chain reaction. See PCR1.
) products. We compared these sequences with all previously documented S-gene sequences of SARS-CoV.

Materials and Methods

Patients and Samples

All patients in the study were hospitalized on our unit with a confirmed diagnosis of SARS. Samples from patients included plasma, throat swab, sputum, and stool; these were stored at--70[degrees]C for extraction of viral RNA. A total of 64 RNA samples from 28 SARS-CoV positive patients (detected by using BNI BNI Business Network International
BNI Business Networking International
BNI Bank Negara Indonesia
BNI Bechtel National, Inc.
BNI British Nursing Index
BNI Barrow Neurological Institute (Phoenix, AZ) 
 primers recommended by the World Health Organization [15]) were initially used in S-gene amplification, but only those that generated all six overlapping fragments covering the full-length S-gene sequence (see Nested RT-PCR below and Figure 1) were included in the sequence analysis. As a result, 29 RNA samples from 20 patients were included in the study (Table 1). All patients had received ribavirin ribavirin /ri·ba·vi·rin/ (ri?bah-vi´rin) a broad-spectrum antiviral used in the treatment of severe viral pneumonia caused by respiratory syncytial virus, particularly in high-risk infants; also used in conjunction with interferon  and steroid combination therapy.

[FIGURE 1 OMITTED]

RNA Extraction

RNA extraction was performed in a biosafety level biosafety level Epidemiology A classification for the degree of caution required when working with specific groups of pathogens. See Maximum containment facility.  3 (P3) laboratory. RNA was extracted directly from plasma samples. Sputum samples were shaken for 30 min with an equal volume of 1.0% acetylcysteine and 0.9% sodium chloride sodium chloride, NaCl, common salt. Properties


Sodium chloride is readily soluble in water and insoluble or only slightly soluble in most other liquids. It forms small, transparent, colorless to white cubic crystals.
, followed by isolating supernatant supernatant /su·per·na·tant/ (-na´tant) the liquid lying above a layer of precipitated insoluble material.

supernatant

the liquid lying above a layer of precipitated insoluble material.
 by centrifuging (10,000 g x 3 min). Throat swab and stool samples were suspended with phosphate-buffered saline (PBS PBS
 in full Public Broadcasting Service

Private, nonprofit U.S. corporation of public television stations. PBS provides its member stations, which are supported by public funds and private contributions rather than by commercials, with educational, cultural,
) containing 10 U/mL RNasin (Promega, Madison, WI) and shaken for 10 min, followed by isolating supernatant by centrifuging as mentioned above. RNA was extracted according to according to
prep.
1. As stated or indicated by; on the authority of: according to historians.

2. In keeping with: according to instructions.

3.
 the manufacturer's instructions by using the QIAamp Viral RNA Mini Kit (Qiagen, Hilden, Germany).

Nested RT-PCR

Screening RNA for SARS-CoV was based on the method by Drosten et al. (1). For the S-gene amplification, 18 pairs of primers were designed by using MacVactor computer software (Accelrys Inc, San Diego San Diego (săn dēā`gō), city (1990 pop. 1,110,549), seat of San Diego co., S Calif., on San Diego Bay; inc. 1850. San Diego includes the unincorporated communities of La Jolla and Spring Valley. Coronado is across the bay. , CA) based on the BJ01 strain of SARS-CoV (GenBank accession no. AY278488) (16). Among them, six pairs (sense/amisense: S1aF/S1aB, S2aF/S2aB, S3aF/S3aB, S4aF/S4aB, S5aF/S5aB, S6aF/S6aB) were used as outer primers, six pairs (sense/antisense: S1bF/S1bB, S2bF/S2bB, S3bF/S3bB, S4bF/S4bB, S5bF/S5bB, S6bF/S6bB) were used as inner primers, and six pairs (sense/antisense: S1cF/S1cB, S2cF/S2cB, S3cF/S3cB, S4cF/S4cB, S5cF/S5cB, S6cF/S6cB) were designed fur direct RT-PCR product sequencing. The sequences covering the full-length S gene were amplified separately as six overlapping fragments (F1b, F2b, F3b, F4b, F5b, and F6b) (Figure 1). The one-step RT-PCR Kit (Qiagen) was used for reverse transcription reverse transcription
n.
The process by which DNA is synthesized from an RNA template.
 and the first round of PCR PCR polymerase chain reaction.

PCR
abbr.
polymerase chain reaction


Polymerase chain reaction (PCR) 
 amplification with outer primers. Thermal cycling consisted of 50[degrees]C for 30 min; 95[degrees]C for 15 min; 10 cycles of 95[degrees]C for 30 s, 57.5[degrees]C for 30 s (decreasing by 1.5[degrees]C every other cycle), 72[degrees]C for 1 min; 40 cycles of 95[degrees]C for 30 s, 54[degrees]C for 30 s, 72[degrees]C for 1 min. Afterwards, 2 [micro]L of the product was used as a template for the second round of PCR amplification in 100-[micro]L volume with inner primers with Taq DNA polymerase DNA polymerase /DNA po·lym·er·ase/ (pah-lim´er-as) any of various enzymes catalyzing the template-directed incorporation of deoxyribonucleotides into a DNA chain, particularly one using a DNA template.  (MBI MBI Management Buy-In
MBI Moody Bible Institute
MBI Mathematical Biosciences Institute
MBI Modular Building Institute
MBI Mechanical Breakdown Insurance
MBI Molecular Biology Institute
MBI Maslach Burnout Inventory (psychometrics) 
 Fermentas, Hanover, MD). Thermal cycling consisted of 30 cycles of 95[degrees]C for 25 s, 54[degrees]C for 25 s, 72[degrees]C for 50 s. In some cases, superScript Any letter, digit or symbol that appears above the line. For example, 10 to the 9th power is written with the 9 in superscript (109). Contrast with subscript.  III RNase Reverse Transcriptase Reverse transcriptase

Any of the deoxyribonucleic acid (DNA) polymerases present in particles of retroviruses which are able to carry out DNA synthesis using an RNA template.
 (Invitrogen, Carlsbad, CA) was used for reverse transcription, according to the manufacturer's instructions. The next two rounds of PCR amplification were performed by using Platinum Pfx DNA Polymerase with a higher fidelity (Invitrogen). The reaction condition was set as above, with a twofold elongation at 68[degrees]C instead of 72[degrees]C. All reactions were carefully carried out to avoid contamination.

TA-Cloning

RT-PCR products were purified by QIAquick PCR Purification Kit (Qiagen) or QIAquick Gel Extraction In molecular biology, gel extraction or gel isolation is a technique used to isolate a desired fragment of intact DNA from an agarose gel following agarose gel electrophoresis.  Kit (Qiagen), with a final volume of 30 [micro]L of elution elution /elu·tion/ (e-loo´shun) in chemistry, separation of material by washing; the process of pulverizing substances and mixing them with water in order to separate the heavier constituents, which settle out in solution, from the . The ligation ligation /li·ga·tion/ (li-ga´shun) the application of a ligature.

tubal ligation  sterilization of the female by constricting, severing, or crushing the uterine tubes.
 and transformation were performed according to the manufacturer's instructions by using pGEM-T Vector System II (Promega). Transformants were selected in LB-agar plate containing 100 [micro]g of ampicillin ampicillin (ăm'pĭsĭl`ĭn), a penicillin-type antibiotic that is effective against both gram-negative microorganisms and gram-positive microorganisms such as Escherichia coli. , 100 [micro]g of 5-bromo-4-chloro-3-indolyl [beta]-L-fucopyranoside (X-gal), and 200 [micro]g of isopropylthiogalactoside. Escherichia coli Escherichia coli (ĕsh'ərĭk`ēə kō`lī), common bacterium that normally inhabits the intestinal tracts of humans and animals, but can cause infection in other parts of the body, especially the urinary tract.  from white clones was added to 5 mL of LB culture for overnight growing at 37[degrees]C with vigorous shaking. Plasmid was purified by QIAprep Spin Miniprep Kit (Qiagen). The recombinant plasmids for sampling sequence analysis were screened by electrophoresis in 1% agarose agarose

more highly purified form of agar with similar uses to agar and widely used in the separation of nucleic acid fragments.
 containing 0.5/[micro]g/mL of ethidium bromide Ethidium bromide (sometimes abbreviated as EtBr) is an intercalating agent commonly used as a nucleic acid stain in molecular biology laboratories for techniques such as agarose gel electrophoresis. .

Sequencing and DNA Analysis DNA analysis Any technique used to analyze genes and DNA. See Chromosome walking, DNA fingerprinting, Footprinting, In situ hybridization, Jeffries' probe, Jumping libraries, PCR, RFLP analysis, Southern blot hybridization.

For each S-gene fragment, four to six clones were screened. To verify variations, 5-50 additional clones generated from independently prepared, RNA-derived RT-PCR products were sequenced in two to four independent experiments. The cloned plasmids were prepared from different RT-PCR products and were directly sequenced for confirmation. DNA sequences were obtained with the use of an automated ABI Abi (ā`bī) [short for Abijah], in the Bible, King Hezekiah's mother.


(Application Binary Interface) A specification for a specific hardware platform combined with the operating system.
 377 sequencer See MIDI sequencer.

(music) sequencer - Any system for recording and/or playback of music via a programmable memory which stores music not as audio data, but as some representation of notes.
 (Applied Biosystems Applied Biosystems, Inc. (formerly NASDAQ: ABIO) is the original name of a pioneer biotechnology company founded in 1981 in Foster City, California, among the Silicon Valley cities of the southern San Francisco Bay Area.  Inc., Foster City, CA). For cloned plasmids, SP6 and T7 primers were used for two-directional sequencing reactions. For PCR products, specific primers (sense: S1cF-S6cF; antisense antisense, DNA or RNA manipulated in a laboratory so that its components (nucleotides) form a complementary copy of normal, or "sense," messenger RNA (mRNA; see nucleic acid). : S1cB S6cB) were used for two-directional sequencing reactions. Analysis and comparison of nucleotide and amino acid amino acid (əmē`nō), any one of a class of simple organic compounds containing carbon, hydrogen, oxygen, nitrogen, and in certain cases sulfur. These compounds are the building blocks of proteins.  sequences were carried out with the DNASTAR computer software (DNASTAR Inc., Madison, WI). The S gene sequence of BJ01 strain was taken as the reference for variation analysis.

Results

With the designed six pairs of primers, all six overlapping S-gene fragments were amplified by nested RT-PCR from 29 RNA samples. However, most RNA samples initially included in the study, though positive for SARS-CoV with BNI primers, failed to simultaneously generate all six overlapping S-gene fragments and were excluded from further sequence analysis. Disintegration of the virus and low viral load viral load
n.
The concentration of a virus, such as HIV, in the blood.


viral load,
n a measure of the number of virus particles present in the bloodstream, expressed as copies per milliliter.
 in the raw samples likely accounted for these failures.

One hundred and thirteen sequence variations distributed in nine variant sites were identified in analyzed sequences that were compared to the reference BJ01 strain of SARS-CoV. BJ01 is an isolate from a tissue-culture propagated sample (16) and is used as reference strain in other studies (9,10). With the exception of one site (position 21702), other variant sites have not, to our knowledge, been documented in humans. Seven of nine variant sites were nonsynonymous. Figure 2 shows the identified variant sites compared to the reference sequence.

[FIGURE 2 OMITTED]

Discussion

We identified novel variant sites and the coexistence of sequences with and without S-gene substitutions in SARS-CoV. Theoretically, a replicating RNA virus expresses a range of genetic and phenotypic variants and has the potential to generate novel virions, which may be selected in response to environmental pressures. RNA viruses generally tolerate high levels of mutagenesis mutagenesis /mu·ta·gen·e·sis/ (mu?tah-jen´e-sis)
1. the production of change.

2. the induction of genetic mutation.


mu·ta·gen·e·sis
n. pl.
 because of their limited genetic complexity (17). Mutations have the potential to be pathogenic (e.g., giving the virus immunity to neutralizing antibodies, cytotoxic T cells cytotoxic T cell
n.
See killer cell.
, or antiviral drugs Antiviral Drugs Definition

Antiviral drugs are medicines that cure or control virus infections.
Purpose

Antivirals are used to treat infections caused by viruses.
 [18-20]). The dynamics of error copying and sequence decomposition are time-dependent. In HIV HIV (Human Immunodeficiency Virus), either of two closely related retroviruses that invade T-helper lymphocytes and are responsible for AIDS. There are two types of HIV: HIV-1 and HIV-2. HIV-1 is responsible for the vast majority of AIDS in the United States.  infection, for example, one adaptive substitution in the env gene env gene

a gene which encodes a protein precursor for the envelope proteins, found in the retroviral genome.
 occurred every 3.3 months or 25 viral generations, averaging across patients (21).

In our study, a higher variation frequency in the S gene was identified for SARS-CoV compared to previous reports (7-10). This difference may be due to a broader sample collection covering a longer timespan of infection. In addition, since virus isolates were not passaged in culture, the whole mutant repertoire is more likely to be detected, since no reverse mutation occurs in cell culture. Our observation most likely reflected the real situation in vivo in vivo /in vi·vo/ (ve´vo) [L.] within the living body.

in vi·vo
adj.
Within a living organism.



in vivo adv.
. Variations were unlikely to result from Taq polymerase errors, since we repeated the experiments for all variations from preparing independent RNA and RT-PCR products and used Platinum Pfx DNA polymerase, which has a high fidelity, to confirm the results in some cases. We could not exclude the possibility that some variations were from defective genomes. However, the fact that the variations remained detectable in the sequences from two or three specimens of the same patient, obtained at different times, suggested that these variations might be active and extensible in vivo.

Sequences with and without substitutions (compared to BJ01) were simultaneously detected in the sequences from seven samples, which suggests the existence of SARS-CoV quasispecies. Furthermore, S-gene sequences from different samples collected at different times from the same patient showed similar, but not exactly identical, variation profiles in four participants (patients 4, 5, 6, and 19 in Table 1); this implies that a dynamic mutational process may exist in vivo. Table 2 summarizes the variations occurring in 29 analyzed S-gene sequences from 20 individual SARS patients.

One nonsynonymous change observed at position A1023G is within the heptad repeat (HR) domains, which is thought to be important for virus entry, and previous study on MHV showed that it would have some effect on virus infection (22). At this stage, we cannot rule out the possibility that this change affects the biological outcome of the virus, but further experiments need to be addressed in the near future.

We observed the coexistence of the S-gene sequences with and without substitutions and time-dependent variation profile in some patients. These observations suggest the possible existence of SARS-CoV quasispecies in an acute infection. In this study, however, the limitation of clinical sample collection and difficulty in directly amplifying full-length S gene from raw clinical samples restricted further extensive study for dynamic mutant distributions of the virus. In addition, the sequencing clone number was conditioned by the scale of the project, and this may have led to some minor variant sequences escaping analysis. Another factor possibly affecting the stability of the viral genome is the administration of the antiviral drug ribavirin. That ribavirin enhances mutagensis of RNA viruses has been addressed (23). Therefore, the artificial effect of ribavirin on the SARS-CoV mutant spectrum remains to be clarified.

The genetic variation of SARS-CoV remains limited in relation to many other RNA viruses such as HIV-1, HCV, and MHV. The probable reason is that SARS-CoV only causes an acute, self-limited infection, which may prevent persistent long-term mutant development in vivo as occurs in chronic RNA viral infections. Notably, some modules in the S protein remain conserved, e.g., the fusion-important HR domains. Although some variations may predict changes of protein functional features, no obvious correlation exists between mutation and clinical disease manifestation from the limited data reported here. Instead, the variation profile was closely correlated with epidemiography; e.g., patients 3-8 were infected in one hospital.

In conclusion, we report here some new variant sites in the S gene of SARS coronavirus and possible existence of SARS-CoV quasispecies in some patients, though in limited numbers. This knowledge furthers our understanding of this emerging virus.

Acknowledgments

We thank K.Y. Yuen for his valuable suggestions for this project; and Panyong Mao and Yuanli Mao for providing some of the samples.

The work was supported by Beijing Natural Science Foundation (Number: 7034051), Emergent Foundation for SARS Treatment and Prevention (Number: 03F017), and in part by Sino-UK Collaboration Foundation for SARS Immunopathogenesis Study (Number: H030230100130).
Table 1. Clinical backgrounds of patients and sample collection

Patient no.   Age (y)   Sex (a)   Onset date   Hostitalized date

1               53         M         2/28            3/05
2               32         M         3/08            3/08
3               32         F         3/20            4/04
4               20         M         3/21            4/06
5               33         M         3/28            4/04
6               59         M         3/30            4/06
7               52         M         3/30            4/04
8               59         M         3/30            4/06
9               19         F         4/01            4/12
10              73         M         4/02            4/03
11              45         F         4/04            4/04
12              26         M         4/08            4/18
13              31         M         4/08            4/14
14              32         M         4/09            4/18
15              39         M         4/10            4/10
16              31         F         4/10            4/12
17              46         F         4/20            4/21
18              48         M         4/20            4/22
19              38         M         4/22            4/26
20              27         M         5/10            5/11

Patient no.   Specimen no. (b)   Sampling date

1                   SW6              3/06
2                   SW17             3/09
3                   PL1              4/07
4                   PL10             4/07
                    PL17             4/22
                    SP4              5/03
5                   PL9              4/07
                    SP1              4/07
6                   PL5              4/07
                    SP9              5/12
7                   PL7              4/07
8                   PL8              4/07
9                   PL15             4/22
                    SP32             4/26
10                  PL6              4/07
                    SP62             4/18
                    SW73             4/21
11                  SP67             4/18
12                  SW76             4/21
13                 ST123             4/26
14                  PL57             4/21
                    SW77             4/22
15                  SP61             4/18
16                  PL59             4/30
17                  SP28             4/26
18                  SP43             4/24
19                  SP13             5/03
                   ST158             4/30
20                  SP8              5/12

(a) M, male; F, female.

(b) First two letters indicate source of sample:
SW, throat swab: PL, plasma; SP, sputum; ST, stool.

Table 2. Variation in S-gene sequences from 20 individual
SARS patients (a,b)

                            21494               21702
Pt. no.   Samp. no.   C [right arrow] T   A [right arrow] G

1            SW6              -                   -
2           SW17           9/2 (c)                +
3            PL1            8/39                8/43
4           PL10            14/7                  +
            PL17              +                   +
             SP4              -                   +
5            PL9              +                   +
             SP1              -                   +
6            PL5              -                   +
             SP9              -                   +
7            PL7              -                   +
8            PL8            7/28                  +
9           SP15              -                   +
            SP32              -                   +
10           SP6              -                   -
            SP62              -                   -
            SW73              -                   -
11          SP67              -                   +
12          SW76              -                   +
13          ST123             -                   +
14          PL57              -                   +
            SW77              -                   +
15          SP61              -                   +
16          PL59              -                   -
17          SP28              -                   +
18          SP43              -                   +
19          ST158             -                   +
            SP13            19/4                14/10
20           SP8              -                   +

                            21858               22908
Pt. no.   Samp. no.   A [right arrow] T   A [right arrow] G

1            SW6              -                   -
2           SW17              -                   -
3            PL1            48/2                  +
4           PL10              -                   +
            PL17              -                   -
             SP4              -                   +
5            PL9              -                   +
             SP1              -                   +
6            PL5              -                   +
             SP9              -                   +
7            PL7              -                   +
8            PL8            33/2                  +
9           SP15              -                   -
            SP32              -                   -
10           SP6              -                   -
            SP62              -                   -
            SW73              -                   -
11          SP67              -                   -
12          SW76              -                   -
13          ST123             -                   -
14          PL57              -                   -
            SW77              -                   -
15          SP61              -                   -
16          PL59              -                   -
17          SP28              -                   -
18          SP43              -                   -
19          ST158             -                   +
            SP13            10/13                 +
20           SP8              -                   -

                            23198               24018
Pt. no.   Samp. no.   T [right arrow] C   A [right arrow] T

1            SW6              -                   -
2           SW17              -                   -
3            PL1              +                   +
4           PL10              +                  2/8
            PL17              -                   +
             SP4              -                   +
5            PL9              +                   +
             SP1              +                   -
6            PL5              +                  8/4
             SP9              +                   +
7            PL7              +                  4/6
8            PL8              +                   +
9           SP15              -                   -
            SP32              -                   -
10           SP6              -                   -
            SP62              -                   -
            SW73              -                   -
11          SP67              -                   -
12          SW76              -                   -
13          ST123             -                   -
14          PL57              +                   +
            SW77              +                   +
15          SP61              -                   -
16          PL59              -                   -
17          SP28              -                   -
18          SP43              -                   -
19          ST158             +                   +
            SP13              +                   +
20           SP8              -                   -

                            24247               24469
Pt. no.   Samp. no.   T [right arrow] C   A [right arrow] G

1            SW6              -                   -
2           SW17              +                   -
3            PL1              +                   +
4           PL10              +                   +
            PL17              +                   +
             SP4              +                   +
5            PL9              +                   +
             SP1              +                   +
6            PL5              +                   +
             SP9              +                   +
7            PL7              +                   +
8            PL8              +                   +
9           SP15              -                   -
            SP32              -                   -
10           SP6              -                   -
            SP62              -                   -
            SW73              -                   -
11          SP67              -                   -
12          SW76              -                   -
13          ST123             -                   -
14          PL57              +                   +
            SW77              +                   +
15          SP61              -                   -
16          PL59              -                   -
17          SP28              -                   -
18          SP43              -                   -
19          ST158             +                   +
            SP13            6/16                  +
20           SP8              -                   -

                            24540
Pt. no.   Samp. no.   A [right arrow] G

1            SW6              -
2           SW17              -
3            PL1              +
4           PL10              +
            PL17              +
             SP4              +
5            PL9              +
             SP1              +
6            PL5              +
             SP9              +
7            PL7              +
8            PL8              +
9           SP15              -
            SP32              -
10           SP6              -
            SP62              -
            SW73              -
11          SP67              -
12          SW76              -
13          ST123             -
14          PL57              +
            SW77              +
15          SP61              -
16          PL59              -
17          SP28              -
18          SP43              -
19          ST158             +
            SP13            14/8
20           SP8              -

(a) The results were determined by analysis of cloned sequences;
+ represents that nucleotide substitution at the variant site is
detected - and represents that the nucleotide at the site is
identical to the one of BJ01 reference sequence in all analyzed
sequences.

(b) SARS, severe acute respiratory syndrome; SW, throat swab;
PL, plasma; SP, sputum; ST, stool.

(c) The numbers represent the ratio of reference to variant
nucleotide detected at the site from the analyzed cloned sequences.


References

(1.) Drosten C, Gunther S, Preiser W, van der Werf S, Brodt HR, Becker S, et al. identification of a novel coronavirus in patients with severe acute respiratory syndrome Severe Acute Respiratory Syndrome (SARS) Definition

Severe acute respiratory syndrome (SARS) is the first emergent and highly transmissible viral disease to appear during the twenty-first century.
. N Engl J Med 2003;348:1967-76.

(2.) Ksiazek TG, Erdman D, Goldsmith CS, Zaki SR, Peret T, Emery S, et al. A novel coronavirus associated with severe acute respiratory syndrome. N Engl J Med 2003;348:1953-66.

(3.) Marra MA, Jones SJ, Astell CR, Holt RA, Brooks-Wilson A, Butterfield YS, et al. The genome sequence of the SARS-associated coronavirus. Science 2003;300:1399-404.

(4.) Liang WN, Mi J, Information Branch Joint Leadership Group of SARS Prevention and Control in Beijing. Epidemiological features of severe acute respiratory syndrome in Beijing. Zhonghua Liu Xing Bing Xue Za Zhi 2003;24:1096-9.

(5.) Domingo E. Quasispecies and the development of new antiviral antiviral /an·ti·vi·ral/ (-vi´ral) destroying viruses or suppressing their replication, or an agent that so acts.

an·ti·vi·ral
adj.
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Dr. Xu is an associate professor of medicine at the Beijing Institute of Infectious Diseases. His work focuses on cancer gene therapy, medical viral molecular biology molecular biology, scientific study of the molecular basis of life processes, including cellular respiration, excretion, and reproduction. The term molecular biology was coined in 1938 by Warren Weaver, then director of the natural sciences program at the Rockefeller , and immunology.

Address for correspondence: Fu Sheng Wang, Beijing Institute of Infectious Diseases, 302 Hospital, 100 Xi Si Huan Middle Road, Beijing 100039, China; tax: 86-10-63831870; email: fswang@public.bta.net.cn

Dongping Xu, * Zheng Zhang, * Fuliang Chu, * Yonggang Li, * Lei Jin, * Lingxia Zhang, * George F. Gao, ([dagger]) and Fu-Sheng Wang *

* Beijing 302 Hospital, Beijing, China; and ([dagger]) University of Oxford, Headington, Oxford, United Kingdom
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Title Annotation:Research
Author:Wang, Fu-Sheng
Publication:Emerging Infectious Diseases
Geographic Code:9CHIN
Date:May 1, 2004
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