More on Mycoplasma
http://www.raintree-health.co.uk/cgi-bin/getpage.pl?/ailments/indicateA.html
Emerging Infectious Diseases. Volume 3. Number 1. January-March 1997
Synopses Mycoplasmas: Sophisticated, Reemerging, and Burdened by Their Notoriety.
Joel B. Baseman and Joseph G. Tully.
The University of Texas Health Science Center at San Antonio, San Antonio,
Texas, USA;
National Institute of Allergy and Infectious Diseases,
Frederick Cancer Research and Development Center, Frederick, Maryland, USA.
"Sit down before fact as a little child, be prepared to give up every
preconceived notion, follow humbly wherever and to whatever abysses nature
leads, or you shall learn nothing."
Thomas Henry Huxley
(More information is available on Mycoplasmas on the Fibromyalgia Link
Mycoplasmas are most unusual self-replicating bacteria, possessing very small
genomes, lacking cell wall components, requiring cholesterol for membrane
function and growth, using UGA codon for tryptophan, passing through
"bacterial-retaining" filters, and displaying genetic economy that
requires a strict dependence on the host for nutrients and refuge. In addition,
many of the mycoplasmas pathogenic for humans and animals possess extraordinary
specialized tip organelles that mediate their intimate interaction with
eucaryotic cells. This host-adapted survival is achieved through surface
parasitism of target cells, acquisition of essential biosynthetic precursors,
and in some cases, subsequent entry and survival intracellularly.
Misconceptions concerning the role of mycoplasmas in disease pathogenesis can
be directly attributed to their biological subtleties and to fundamental
deficits in understanding their virulence capabilities. In this review, we
highlight the biology and pathogenesis of these procaryotes and provide new
evidence that may lead to increased appreciation of their role as human
pathogens.
No other group of procaryotes has been so embroiled in controversy and in
establishing a clear pathogenic niche as the mycoplasmas. Their virulence
determinants are undeniably complex, and their unique biological properties
likely challenge the host differently from typical bacterial pathogens (1,2).
Also, numerous Mycoplasma species appear to comprise the commensal microbial
flora of healthy persons (3), and the association of these mycoplasmas with
disease complicates the diagnosis and necessitates extensive and highly
specific serologic, nucleic acid, and epidemiologic data. Nonetheless,
mycoplasmas by themselves can cause acute and chronic diseases at multiple
sites with wide-ranging complications and have been implicated as cofactors in
disease. Recently, mycoplasmas have been linked as a cofactor to AIDS
pathogenesis and to malignant transformation, chromosomal aberrations, the Gulf
War Syndrome, and other unexplained and complex illnesses, including chronic
fatigue syndrome, Crohn's disease, and various arthritides (4-8). Even with
mounting evidence of their pervasive and pathogenic potential, mycoplasmas
still evoke the image of a group of obscure or impotent microorganisms. Yet
they are evolutionarily advanced procaryotes (9-11), and their elite status as "next
generation" bacterial pathogens necessitates new paradigms in fully
understanding their disease potential.
Mycoplasmas, which lack cell walls but possess distinctive sterol-containing
plasma membranes, are taxonomically separated from other bacteria and belong to
the class Mollicutes (mollis, soft; cutis, skin). Mollicutes, a term that
includes the cell wall-less procaryotes assigned to numerous genera under the
class Mollicutes and is frequently used interchangeably with mycoplasmas, are
unusual for other biological reasons as well. They are evolutionary descendants
of the low G+C containing gram-positive bacteria and, through chromosome
reduction, represent the smallest self-replicating life forms. Their
streamlined genome size, which illustrates extreme biological gene economy,
imposes complex nutritional requirements, such as dependence on external
supplies of biosynthetic precursors, including amino acids, nucleotides, fatty
acids, and sterols. This limited coding capacity dictates for mycoplasmas a
parasitic way of life that few pathogenic micro-organisms can claim. Therefore,
the view that pathogenic mycoplasmas can grow "independently"
requires an appreciation of their fastidious nature and their intimate
dependence upon the host. Because of these properties, pathogenic mycoplasmas
are among the most difficult micro-organisms to grow from clinical specimens
and remain frequent contaminants of primary and continuous eucaryotic cell
lines and tissue cultures (12). In some instances, mycoplasma contamination is
obvious since infected eucaryotic cells exhibit aberrant growth, metabolism,
and morphology. However, mycoplasmas often establish covert and chronic
infections of target cells that lead to either invalid and misleading data or
introduction of mycoplasmas or their products into reagents dedicated to
therapeutic or research purposes. The recent emphasis on isolating viral
agents, such as human immunodeficiency virus (HIV)-1, from human primary
lymphocytic cells has also demonstrated the frequent cocultivation of
mycoplasmas of human origin. Often, the unwanted sources of exogenous
mycoplasmas are serum products and filter-"sterilized"(450 nm)
solutions; cross-contamination by already infected cell cultures, viral stocks,
or immunologic preparations; breaks in technique, including aerosols from the
respiratory tract or by mouth pipetting; ignorance of the mycoplasma problem;
or scientific indifference.
Detailed up-to-date reviews describing the biological and pathogenic properties
of mycoplasmas have been published (1,2,13,14). Our intention here is to
provide a concise historical perspective of the role of mycoplasmas in human
disease; highlight the discoveries of new Mycoplasma species and their
association with human illness and host conditions that present problems in
detection and treatment; describe selected biological properties of mycoplasmas
consistent with their intimate host relationship and possible mechanisms of
pathogenicity; and address recent controversies associated with mycoplasmas as
emerging infectious agents. Renewed attention to these issues may provide the
impetus to demystify mycoplasmas and improve their standing as genuine,
card-carrying pathogens.
Historical Perspectives
The earliest reports of mycoplasmas as infectious agents in humans appeared in
the 1930s and 1940s. At that time, primary atypical pneumonia was associated
with an infectious agent that because of its minute size and innate biological
properties unknown at that time, passed through bacteria-retaining filters,
resisted penicillin and sulfonamide therapies, and adapted to growth in
embryonated eggs and tissue culture cells. Correlations between the etiologic
agent of "walking pneumonia" with viruses, L-forms, and
pleuropneumonia-like agents (referred to as PPLOs in publications and textbooks
of that era) were frequent and often misleading. Finally, definitive studies in
the early 1960s established Mycoplasma pneumoniae as the singular cause of cold
agglutinin-associated primary atypical pneumonia (2). Today M. pneumoniae
remains an important cause of pneumonia and other airway disorders, such as
tracheobronchitis and pharyngitis (13,14), and is associated with
extrapulmonary manifestations, such as hematopoietic, exanthematic, joint,
central nervous system, liver, pancreas, and cardiovascular syndromes (15).
The confusion associated with M. pneumoniae-mediated infections has recurred
many times with other mycoplasmas, whose detection in clinical specimens
through culture, antibody, or DNA-based testing is frequently dismissed as
"only mycoplasmas" even when they appear to be the primary pathogens.
Two mycoplasmas commonly found in the urogenital tracts of healthy persons are
Mycoplasma hominis and Ureaplasma urealyticum. However, over the years, the pathogenic
roles of these mycoplasmas have been proven in adult urogenital tract diseases,
neonatal respiratory infections, and a range of other diseases usually in
immunocompromised patients (2).
Several recent examples illustrate the increasing impact of Mycoplasma species
on emerging diseases. Mycoplasma fermentans strains were first isolated from
the lower genital tract of both adult men and women in the early 1950s, but
their role in classic lower genital tract disease has not been established
(16). Reports in the 1970s of M. fermentans in the joints of rheumatoid
arthritis patients and in the bone marrow of children with leukemia raised
expectations for its pathogenic potential (17,18); these findings have not been
adequately confirmed. Sufficient evidence, however, has accumulated recently to
establish an important and emerging role for M. fermentans in human respiratory
and joint diseases. For example, M. fermentans has been detected by specific
gene amplification techniques such as polymerase chain reaction (PCR) in the
synovial fluid of patients with inflammatory arthritis, but not in the joints
of patients with juvenile or reactive arthritis (19). In two other studies
using PCR, M. fermentans was identified in the upper respiratory tract of 20%
to 44% of both healthy and HIV-infected patients (20,21) and was associated
with acute respiratory distress syndrome in nonimmunocompromised persons (22).
Mycoplasma genitalium was detected in the urogenital tract of two patients with
nongonococcal urethritis in 1981 (23), but for more than a decade, very little
was known about its host distribution and pathogenicity. Early experimental
studies established that the organism caused lower genital tract infections in
both male and female chimpanzees, with extensive urethral colonization in males
and apparent tissue invasion, eventually leading to overt bacteremia (24).
However, the fastidious growth requirements of M. genitalium from human hosts
severely limited further study until the advent of molecular detection techniques.
Specific sequences in the 140 kDa adhesin protein gene of M. genitalium were
selected as targets in a PCR-based detection assay (25,26). Subsequent
application of these techniques in cases of acute nongonococcal urethritis, not
including those of patients colonized or infected with Chlamydia trachomatis,
has provided mounting evidence for the involvement of M. genitalium as an
etiologic agent of this disease (27-29). Also, M. genitalium has been suspected
in chronic nongonococcal urethritis and pelvic inflammatory disease (30).
The discovery in 1988 of M. genitalium strains in human nasopharyngeal throat
specimens, where they were frequently mixed with strains of M. pneumoniae, not
only changed dramatically the concept of host distribution of M. genitalium but
also prompted critical questions about the role of this mycoplasma in human
respiratory disease (31). However, the immunologic cross-reactivity between M.
genitalium and M. pneumoniae and the inability of most conventional diagnostic
serologic tests to conclusively identify M. genitalium have complicated its
delineation in acute human respiratory disease. PCR assays specific for the
organism have detected M. genitalium in throat specimens of patients infected
with HIV-1 (32). However, these probes have not been applied to control groups
and patients in outbreaks of acute respiratory disease and/or pneumonia to
determine whether M. genitalium alone is an etiologic agent in respiratory
infections.
M. genitalium has been implicated as an etiologic agent in certain human joint
diseases. This clinical correlation began with the observation of a mixed
infection of M. pneumoniae and M. genitalium in synovial fluid specimens of a
nonimmunocompromised patient after an acute respiratory infection (33). A predominant
role was not established for either Mycoplasma species in the initial
respiratory disease or in the joint manifestations, although evidence to
implicate postinfectious autoimmunity to both organisms was described. These
findings prompted a PCR assay on synovial fluids from patients with various
arthritic syndromes, which presented case reports on two of 13 patients with M.
genitalium detected in joint fluids (34).
Another area of emerging mycoplasmal infections concerns immunodeficiency.
Although patients with congenital or acquired disorders of antibody production
are susceptible to a wide variety of microbial infections, the unique
susceptibility of such patients to mycoplasmal infections is a growing concern,
especially considering the number of occurrences, the types of mycoplasmas
involved, and the difficulties posed in the therapeutic management of such
infections. In addition, the increased use of prolonged or permanent
immunosuppressive chemotherapy required for patients undergoing tissue or organ
transplantation or treatment of various malignant diseases has also increased
the risk for mycoplasmal infections from mycoplasmas that are part of the
normal human mollicute flora to those acquired through animal contact.
The association between immunodeficiency and mycoplasmal infections was first
reported in the mid 1970s in patients with primary hypogammaglobulinemia and
infection with U. urealyticum, M. pneumoniae, Mycoplasma salivarium, and M.
hominis that localized in joint tissue, frequently with destructive arthritis.
Similar joint infections in hypogammaglobulinemic patients with these
mycoplasmal species continue to be reported (35). Since most of these
mollicutes, with the possible exception of M. pneumoniae, occur as part of the
normal human flora, the origin of such joint infections is considered
endogenous. Patients with hypogammaglobulinemia and other antibody deficiencies
are also especially susceptible to mycoplasmal infections of the upper
respiratory and urinary tracts caused most frequently by M. pneumoniae or U.
urealyticum, respectively (36).
Mycoplasmal infections following organ transplantation and immunosuppressive
chemotherapy were observed in the early 1980s, with both M. hominis and U.
urealyticum reported most often (37-39). Although these infections most likely
originated from the patient's normal microbial flora, a recent report of donor
transmission of M. hominis to two lung allograft recipients (40) suggests that
donor tissue may be a more important factor in transplant infections than
currently recognized.
While patients with antibody defects or those receiving immunosuppressive drugs
appear to be the most susceptible to infections with mycoplasmas present in
healthy tissues, emerging evidence indicates that contact with other
mycoplasmas in the environment is an important hazard. For example, the direct
isolation of a feline mycoplasma (M. felis) from the joint of a
hypogammaglobulinemic patient with septic arthritis was recently reported (41),
with suspected transmission occurring through a cat bite 6 months before the
onset of arthritis. Other examples include fatal septicemia caused by M.
arginini, a common animal mycoplasma, from blood and multiple tissue sites in a
slaughter house employee who had advanced non-Hodgkin's lymphoma and
hypogammaglobulinemia (42), and a septicemic infection with a canine mycoplasma
(M. edwardii) in a patient with advanced AIDS (M.K.York, pers. comm.).
One of the most critical aspects of mycoplasmal infections in immunodeficient
patients is the frequent inability to control such infections with appropriate
broad spectrum antibiotics. Although the tetracyclines and erythromycins are
effective chemotherapeutic agents for many mycoplasmal infections, M.
fermentans and M. hominis strains are usually resistant to erythromycin, and
tetracycline-resistant strains of M. hominis andU. urealyticum have been
reported from the lower urogenital tract of patients. However, these
antibiotics and most other broad spectrum agents have limited mycoplasmacidal
activity in vivo, and their efficacy eventually depends on an intact host
immune system to eliminate the mycoplasmas. Most hypogammaglobulinemic patients
lack the ability to mount a strong antibody response. Guidelines for managing
such mycoplasmal infections in patients with immune defects should include
immediate in vitro testing of the isolated mollicute against a wide range of
antibiotics; expeditious administration of the antibiotic by the most
appropriate route (intravenously, if warranted); prolonged therapy terminated
only if there is no rapid clinical or microbiological response; and possibly
administration of intravenous immunoglobulin (35,36). Clinical management of
mycoplasmal infections in transplant patients is more difficult since immunoglobulins
may enhance graft or organ rejection. In the absence of suitable
mycoplasmacidal chemotherapeutic agents, vigorous and sustained chemotherapy
with the most active antibiotic is the current method of choice.
Mechanisms of Pathogenicity.
Many mycoplasmal pathogens exhibit filamentous or flask-shaped appearances and
display prominent and specialized polar tip organelles that mediate attachment
to host target cells (43,44). These tip structures are complex, composed of a
network of interactive proteins, designated adhesins, and adherence-accessory
proteins (Figure 1, [14,43]). These proteins cooperate structurally and
functionally to mobilize and concentrate adhesins at the tip and permit
mycoplasmal colonization of mucous membranes and eucaryotic cell surfaces,
probably through host sialoglycoconjugates and sulfated glycolipids (Figure 2,
[14,43,45]). It appears that mycoplasmal cytadherence-related proteins
represent a superfamily of genes and proteins that have been conserved through
horizontal gene transfer from an ancestral gene family. This protein network
resembles a specialized cytoskeleton-like apparatus, which may represent the
precursor to mammalian cytoskeletal and extracellular matrix-like complexes
(14). Other Mycoplasma species lack distinct tip structures yet are capable of
cytadherence, and they may use related genes or proteins or alternative
mechanisms of surface parasitism.
[Figure 1] [Figures not available in ASCII version] Figure 1. Transmission
electron photomicrographs of the specialized tip organelle of
cytadherence-positive M. pneumoniae demonstrating a) truncated structure with
nap, b) clustering of cytadherence-related proteins (P1, B, C, P30) at the tip
based on immunolabeling with ferritin and colloidal gold and crosslinking studies,
and c) Triton X-100-resistant, cytoskeleton-like, structure with distinct bleb
and parallel filaments (14,43,45,46).
[Figure 2] [Figures not available in ASCII version] Figure 2. Transmission
electron photomicrograph of a hamster trachea ring infected with M. pneumoniae
(43). Note the orientation of the mycoplasmas through their specialized tiplike
organelle, which permits close association with the respiratory epithelium. M,
mycoplasma; m, microvillus; C, cilia.
The family of mycoplasmal genes and proteins involved in cytadherence has been
studied most extensively in M. pneumoniae (14,43,46-48). Noncytadhering
phenotypes that arise through spontaneous mutation at high frequency have been
categorized into mutant classes on the basis of distinct protein profiles.
These noncytadhering mycoplasmas cannot synthesize specific
cytadherence-related proteins or are unable to stabilize them at the tip
organelle, which leads to abnormal anatomical tip structures and avirulence
(43). Spontaneous reversion to the cytadhering phenotype is accompanied by the
reappearance of the implicated proteins, restoration of structurally and
functionally intact tips, and return of full infectivity (43). Similar
cytadherence-related genes and proteins have been reported for M. genitalium on
the basis of biochemical, immunologic, and genetic analyses (25,49,50).
Furthermore, striking similarities exist in the order of operons that comprise
the cytadherence-related genes and the organization of these genes within each
operon of M. pneumoniae and M. genitalium (14,50,51). These similarities
reinforce the unexpected coisolations of M. genitalium, along with M.
pneumoniae, from the nasopharyngeal throat swabs of patients with acute
respiratory diseases and from synovial fluids of patients with arthritis as
described in the previous section (31,33). The isolation of M. pneumoniae from
the human urogenital tract (52) further suggests that these mycoplasmas have
evolved parasitic strategies that include overlapping tissue tropisms as determined
by the genetic and chemical relatedness of their cytadherence genes and
proteins (14,25,43,50,51). The recent use of transposon mutagenesis to generate
M. pneumoniae and M. genitalium transformants displaying cytadherence-deficient
phenotypes should further clarify the relationships between the
cytadherence-related genes and proteins and identify additional sites
previously unlinked to cytadherence (46,53).
An interesting feature of specific M. pneumoniae and M. genitalium adhesins is
their multiple gene copy nature (14,43,54,55,56). Although only one full-length
copy of the adhesin structural genes exists in adhesin-related operons, precise
regions of these adhesin genes are detected as single genomic copies, while
other regions occur as closely homologous, but not identical, multiple copies.
In other words, multiple truncated and sequence-related copies of the adhesin
genes are dispersed throughout the genome, which could generate adhesin
variation through homologous recombination. Consistent with this possibility is
the existence of restriction fragment length polymorphisms in the adhesin genes
of human clinical isolates of M. pneumoniae and M. genitalium, reflected by
sequence divergence in the multiple-copy regions of the adhesin genes (56-59).
It appears that a repertoire of partial adhesin-related gene regions serves as
a reservoir to regulate the structural and functional properties of mycoplasmal
adhesins through recombination events, which may lead to circumvention of the
host immune response. Mechanisms of phase and antigenic variation are likely to
occur in which mycoplasmal adhesins exhibit altered specificities and
affinities, as determined by the organization of constant and variable adhesin
gene sequences. Therefore, despite their small genomes, pathogenic mycoplasmas
facilitate DNA rearrangements through repetitive gene sequences, thus promoting
genetic diversity and maximizing the coding potential of their limited genomes.
The immunodominant epitopes of the mycoplasmal adhesins appear not to be
identical to the adherence-mediating domains (13). The latter are in part
encoded by single copy regions of the adhesin genes and are highly conserved,
which reinforces their essential role in mycoplasmal recognition of host cell
receptors and colonization (60,61). Host immunoresponsiveness directed at the
noncytadherence-mediating variable regions is unlikely to generate effective
cytadherence-blocking antibodies, which may in part clarify the observed high
reinfection rates of patients. Thus, the grouping of clinical isolates of M.
pneumoniae into two categories, on the basis of sequence divergence in the
multiple-copy regions of the adhesin gene (56-59), along with the immune status
of the population, may explain the epidemiologic patterns of M. pneumoniae
reported over the years.
Another characteristic of the cytadherence-related proteins is their
proline-rich composition, which markedly influences protein folding and
binding. Several reports have established the importance of these proline-rich
domains in mycoplasmal cytadherence and virulence (47,48,62,63), and recent
evidence further suggests that mycoplasmal peptidylprolyl isomerases, i.e.,
cyclophilins, are critical in regulating the conformation and function of the
mycoplasmal cytadherence-related tip organelle, colony morphology, and growth
(14,64). In addition to this proline-rich property, one of the most unusual
features of the adhesins is their extensive sequence homology to mammalian
structural proteins (1,14,33,43,47,48). This molecular mimicry is especially
interesting since it has been suggested for decades that mycoplasmas provoke an
antiself response that triggers immune disorders, although the basis for the
induction has been elusive (65). Patients with documented M. pneumoniae respiratory
infections demonstrate seroconversion to myosin, keratin, and fibrinogen (33)
and exhibit extrapulmonary manifestations, such as exanthems and cardiac
abnormalities. Furthermore, a classic example of bacteria-mediated autoimmune
disorders is the development of acute rheumatic fever following streptococcal
infection (66). Antistreptococcal antibodies reactive against ahelical
coiled-coil regions of the M protein crossreact with heart myosin, tropomyosin,
and mycoplasmal adhesins (14,66). In the latter case, these mycoplasmal
adhesins exhibit amino acid sequence homologies with human CD4 and class II
major histocompatibility complex lymphocyte proteins, which could generate
autoreactive antibodies and trigger cell killing and immunosuppression (67,68).
Also, mycoplasmas may serve as B-cell and T-cell mitogens and induce autoimmune
disease through the activation of antiself T cells or polyclonal B cells. The
multiorgan protean manifestations of mycoplasmal infections in humans are
consistent with the pathogenesis of autoimmunity. Furthermore, the ability of
mycoplasmas to induce a broad range of immunoregulatory events, mediated by
cytokine production and direct effects on macrophages, B and T cells, and glial
cells, is evidence that mycoplasmas possess the attributes of primary mediators
of pathogenesis (1,2,12,69). For example, cytokine production and lymphocyte
activation may either minimize disease through the activation of host defense
mechanisms or exacerbate disease through lesion development (69,70). Also, a
superantigen derived from Mycoplasma arthritidis, a mycoplasma pathogenic for
rodents, induces arthritis and chronic disease manifestations (69). It has been
suggested that related superantigen-like molecules may exist in mycoplasmas of
human origin triggering autoimmune and other inflammatory pathologies.
It appears that cytadherence is the initial step in the virulence process of
pathogenic mycoplasmas (Figure 2) and precedes a spectrum of subtle or overt
host cell responses. In specific instances, distinct cytopathology correlates
with the infecting Mycoplasma species, the number of adherent mycoplasmas, the
length of coincubation, the induction of proinflammatory cytokines, and the age
and immune status of the patient. For example, the exacerbation of clinical
syndromes may correlate with a history of mycoplasmal infection as observed in
patients with recurrent M. pneumoniae exposures (2,13). Also, the elevated
expression of proinflammatory cytokines associated with mycoplasmal disease
pathogenesis may coincide with the intensity of the symptoms. In other cases,
chronic disease or no obvious signs or symptoms of disease accompany
mycoplasmal infection.
Other biological properties of mycoplasmas have been implicated as virulence
determinants and include 1) generation of hydrogen peroxide and superoxide
radicals by adhering mycoplasmas, which induces oxidative stress, including
host cell membrane damage; 2) competition for and depletion of nutrients or
biosynthetic precursors by mycoplasmas, which disrupts host cell maintenance
and function; 3) existence of capsule-like material and electron-dense surface
layers or structures, which provides increased integrity to the mycoplasma
surface and confers immunoregulatory activities; 4) high-frequency phase and
antigenic variation, which results in surface diversity and possible avoidance
of protective host immune defenses; 5) secretion or introduction of mycoplasmal
enzymes, such as phospholipases, ATPases, hemolysins, proteases, and nucleases
into the host cell milieu, which leads to localized tissue disruption and
disorganization and chromosomal aberrations; and 6) intracellular residence,
which sequesters mycoplasmas, establishes latent or chronic states, and
circumvents mycoplasmicidal immune mechanisms and selective drug therapies
(1,2,71,72). Whether pathogenic mycoplasmas enter and survive within mammalian
cells has been debated for many years. Consistent with this possibility,
mycoplasmas exhibit limited biosynthetic capabilities; are highly fastidious
and dependent upon the host microenvironment and complex culture medium for
growth; have been observed in intimate contact with mammalian cell surfaces and
within target cells; may be capable of initiating fusion with host cells
through their cholesterol-containing unit membranes; and survive long-term
recommended antimicrobial treatment in humans and tissue cultures. Recent
sightings of intact mycoplasmas throughout the cytoplasm and the perinuclear
regions of tissue cells from infected patients and in cell cultures, along with
evidence that mycoplasmas are capable of long-term intracellular survival and
replication in vitro, offer an additional dimension to the pathogenic potential
of mycoplasmas (4,14,72,73).
The Latest Controversies: Food for Thought or the Twilight Zone.
On the basis of the above information, the virulence strategies displayed by
mycoplasmas are likely the summation of a multitude of biological activities
(1). Since no obvious single or group of mycoplasmal properties inextricably
correlates with disease manifestations, the proof that mycoplasmas are
card-carrying pathogens necessitates thorough and highly specific
microbiological, epidemiologic, and diagnostic criteria; detailed descriptions
of biochemical, genetic, and immunologic characteristics that distinguish
virulent and avirulent mycoplasmas; and reproducibility of the symptoms of
disease in experimental animal models or in the natural spread of infection
among susceptible populations. The portfolio of available evidence concerning
mycoplasma-mediated disease pathogenesis is limited. These scientific
shortcomings precipitate misconceptions concerning mycoplasmas as singular
agents of infectious diseases, as putative cofactors in the progression of
other diseases, and as universal contaminants of cell cultures. Clearly,
multiple pathways of interaction with target cells appears to be the modus
operandi of the Mycoplasma species. With this conceptual scientific framework
as a background, five recently proposed and controversial associations of
mycoplasmas to human diseases are worth noting.
AIDS
The role of mycoplasmas in accelerating the progression of AIDS could not have
begun under more baffling and circuitous conditions. A virus-like agent that
arose through transfection of NIH 3T3 cells with DNA from Kaposi sarcoma
tissues of AIDS patients was later shown to be M. fermentans. The spotted
history of M. fermentans in rheumatoid arthritis and leukemia and its frequent
contamination of cell cultures, along with its contemporary link to AIDS, have
been considerable impediments to overcome in its elevation to pathogenic
status. However, careful and convincing independent studies by several
laboratories have implicated M. fermentans as a cause of systemic infections
and organ failure in AIDS patients (4,74). The isolation of M. fermentans from
blood and urine samples of HIV-infected persons, its detection by PCR and
immunohistochemistry in multiple tissue sites at various stages of AIDS, and
its ability to stimulate CD4+ lymphocytes and other immunomodulatory activities
implicate this Mycoplasma species as a cofactor in AIDS. Consistent with this
possibility, M. fermentans has been shown to act synergistically with HIV to
enhance cytopathic effects on human CD4+ lymphocytes. Coincident with these
studies, a new Mycoplasma species, Mycoplasma penetrans, also has emerged as a
potential cofactor in AIDS progression (75,76). Its isolation almost
exclusively from the urine of HIV-infected patients, the extraordinarily high
prevalence of antibodies against this mycoplasma in HIV-infected patients and
not in HIV-seronegative persons, and its capacity to invade target cells and
activate the immune system of HIV-infected patients at various stages of
disease correlate with a synergistic role with HIV. Other mycoplasmas,
including M. genitalium and Mycoplasma pirum, have also been isolated from AIDS
patients and implicated as potential cofactors. However, the proposed role of
mycoplasmas as infectious agents and cofactors in AIDS-related disorders still
remains a hypothesis without definitive proof. If cofactors of HIV are
essential to the development of late stages of HIV-mediated disease,
mycoplasmas possess all the prerequisite properties of the consummate helper.
Their ability to establish covert or overt chronic and persistent infections
with concomitant activation of the immune system, stimulation of cytokine
production, and induction of oxidative stress correlate with increased HIV
replication and disease progression. Are mycoplasmas irrelevant to AIDS, or are
the clinical and microbiological correlations sufficient to imply intimate
relationships between HIV and mycoplasmas, especially as the infected host
undergoes immunologic distress?
Malignant Transformation.
As early as the mid-1960s, mycoplasma-infected cell lines were associated with
chromosomal aberrations, altered morphologies, and cell transformation (77,78).
These abnormal oncogenic cell traits continued even after the apparent
elimination of mycoplasmas, and evidence implied increased tumorigenicity of
these transformed cells in animals. This issue has been revisited in studies
demonstrating that longterm, persistent mycoplasmal infection of mouse embryo
cells initiated a multistage cellular process that resulted in irreversible cell
transformation, karyotypic alterations, and tumorigenicity in nude mice (6). Do
these oncogenic events associated with mycoplasma-mammalian cell coincubation
relate to the ontogeny of human cancers?
Gulf War Syndrome
One of the most controversial current medical issues is whether the multiple
acute and chronic symptoms found in veterans of the Persian Gulf War were
caused by chemical exposure, infectious agents, or psychological problems, or
whether a Gulf War Syndrome exists at all. The clinical illness comprises a
collection of symptoms, including chronic fatigue, joint pain, headaches, and
skin rashes. One study suggests that pathogenic mycoplasmas are responsible for
a large number of cases among veterans, on the basis of DNA hybridization and the
responsiveness of veterans to prolonged antibiotic treatment (5). Even though
the experimental evidence is sparse and incomplete and well-controlled and
detailed studies by independent laboratories are needed, if the Gulf War
Syndrome has infectious causes, mycoplasmas with their requisite biological
credentials are potential candidates.
Crohn's Disease.
Several epidemiologic studies correlate respiratory infections with
exacerbation of Crohn's disease and other chronic inflammatory bowel diseases
(7,79). Acute onset gastrointestinal symptoms in patients with these diseases
are accompanied by seroconversion to specific viral or M. pneumoniae antigens.
As indicated earlier, mycoplasmas can elicit pleiotropic immune responses and
are difficult to eliminate in patients despite appropriate antibiotic
treatment. Steroid therapy to control gastrointestinal symptoms in these
patients, along with the multifaceted biological properties associated with
pathogenic mycoplasmas, may precipitate the onset of acute exacerbations of
chronic inflammatory bowel disease.
Rheumatoid Arthritis and Other Human Arthritides.
The occurrence of various Mycoplasma and Ureaplasma species in joint tissues of
patients with rheumatoid arthritis, sexually transmitted reactive arthritis,
and other human arthritides can no longer be ignored (8). A clinical trial of
longterm (6 to 12 months) antibiotic (doxycycline) therapy before cartilage
destruction might prove beneficial in managing such frequent and often
debilitating infections.
Extensive clinical and microbiological evidence indicates that mycoplasmas
alone can elicit a spectrum of illness for which no other agents are
incriminated. The eradication of these pathogenic mycoplasmas from various
tissue sites requires an intact and functional immune system, although persons
with fully competent immune systems may have difficulty eliminating
mycoplasmas, even with recommended prolonged drug therapy. Nonetheless,
mycoplasmas are still viewed as subordinates to other infectious agents and are
relegated to a category of commensals that unwittingly cause disease in
patients whose immune systems offer little resistance to microbial stress and
overload.
The fundamental importance of mycoplasmas in specific diseases of humans,
animals, insects, and plants is irrefutable, and their unique biological
properties are consistent with their intimate association with host target
cells. These remarkable bacteria must continue to receive the scientific
attention of mycoplasmologists, cell culturists, clinicians, immunologists, and
DNA sequencers who most recently are compiling extensive databases that may
eventually dissect every approachable mycoplasmal element that defines their
biological and genetic being. Nonetheless, mycoplasmas remain mysterious and enigmatic,
and the available data and proposed hypotheses that correlate mycoplasmas with
disease pathogenesis range from definitive, provocative, and titillating to
inconclusive, confusing, and heretical. Controversy seems to be a recurrent
companion of mycoplasmas, yet good science and openmindedness should overcome
the legacy that has burdened them for decades.
Acknowledgments.
This study was supported in part by NIH grants AI 27873, AI 32829 and AI 41010.
Dr. Baseman is professor and chair, Department of Microbiology, University of
Texas Health Science Center, San Antonio. His research focuses on pathogen-host
cell interactions with special interest in defining the biology and virulence
determinants of mycoplasmas pathogenic for humans.
Dr. Tully heads the Mycoplasma Section, Laboratory of Molecular Microbiology,
National Institute of Allergy and Infectious Diseases, Frederick, Maryland. His
interest covers the host distribution, pathogenicity, and taxonomy of
mollicutes.
Address for correspondence: Joel B. Baseman, Department of Microbiology, The
University of Texas Health Science Center at San Antonio, 7703 Floyd Curl
Drive, San Antonio, TX 78284-7758; fax: 210-567-6491; e-mail:
baseman@uthscsa.edu.
References
1. Tryon VV, Baseman JB. Pathogenic determinants and mechanisms. In: Maniloff
J, McElhaney RN, Finch LR, Baseman JB, editors. Mycoplasmas: molecular biology
and pathogenesis. Washington (DC): American Society for Microbiology,
1992:457-71.
2. Krause DC, Taylor-Robinson D. Mycoplasmas which infect humans. In: Maniloff
J, McElhaney RN, Finch LR, Baseman JB, editors. Mycoplasmas: molecular biology
and pathogenesis. Washington (DC): American Society for Microbiology,
1992:417-44.
3. Tully JG. Current status of the mollicute flora of humans. Clin Infect Dis
1993;17:S2-9.
4. Lo S-C. Mycoplasmas and AIDS. In: Maniloff J, McElhaney RN, Finch LR,
Baseman JB, editors. Mycoplasmas: molecular biology and pathogenesis.
Washington (DC): American Society for Microbiology, 1992:525-45.
5. Nicolson G, Nicolson NL. Diagnosis and treatment of mycoplasmal infections
in Gulf War illness-CFIDS patients. Intl J Occup Med Immunol Toxicol
1996;5:69-78.
6. Tsai S, Wear DJ, Shih JW-K, Lo SC. Mycoplasmas and oncogenesis:persistent
infection and multistage malignant transformation. Proc Natl Acad Sci USA
1995;92:10197-201.
7. Ekbom A, Daszak P, Kraaz W, Wakefield AJ. Crohn's disease after in-utero
measles virus exposure. Lancet 1996;348:516-7.
8. Taylor-Robinson D. Mycoplasmas in rheumatoid arthritis and other human arthritides.
J Clin Pathol 1996;49:781-2.
9. Bové JM. Molecular features of mollicutes. Clin Infect Dis 1993;17:S10-31.
10. Razin S. Molecular properties of mollicutes: a synopsis. In: Razin S, Tully
JG, editors. Molecular and diagnostic procedures in mycoplasmology, Vol I. New
York: Academic Press, Inc., 1995:1-25.
11. Dybvig K, Voelker LL. Molecular biology of mycoplasmas. Annu Rev Microbiol
1996;50:25-57.
12. McGarrity GJ, Kotani H, Butler GH. Mycoplasmas and tissue culture cells.
In: Maniloff J, McElhaney RN, Finch LR, Baseman JB, editors. Mycoplasmas:
molecular biology and pathogenesis. Washington (DC): American Society for
Microbiology, 1992:445-54.
13. Jacobs E. Mycoplasma pneumoniae virulence factors and the immune response.
Rev Med Microbiol 1991;2:83-90.
14. Baseman JB, Reddy SP, Dallo SF. Interplay between mycoplasma surface
proteins, airway cells, and the protean manifestations of mycoplasma-mediated
human infections. Am J Respir Crit Care Med 1996;154:S137-44.
15. Murray HW, Masur H, Senterfit LB, Roberts RB. The protean manifestations of
Mycoplasma pneumoniae infection in adults. Am J Med 1975;58:229-42.
16. Deguchi T, Gilroy CB, Taylor-Robinson D. Failure to detect Mycoplasma
fermentans, Mycoplasma penetrans, or Mycoplasma pirum in the urethra of
patients with acute nongonococcal urethritis. Eur J Clin Microbiol Infect Dis
1996;15:169-71.
17. Williams MH, Brostoff J, Roitt IM. Possible role of Mycoplasma fermentans
in pathogenesis of rheumatoid arthritis. Lancet 1970;ii:270-80.
18. Murphy WH, Gullis C, Dabich L, Heyn R, Zarafonetis CJD. Isolation of
Mycoplasma from leukemic and nonleukemia patients. J Nat Cancer Inst
1970;45:243-51.
19. Schaeverbeke T, Gilroy CB, Bébéar C, Dehais J, Taylor-Robinson D.
Mycoplasma fermentans, but not M. penetrans, detected by PCR assays in synovium
from patients with rheumatoid arthritis and other rheumatic disorders. J Clin
Pathol 1996;41:311-4.
20. Katseni VL, Gilroy CB, Ryait BK, Ariyoshi K, Bieniasz PB, Weber JN, et al.
Mycoplasma fermentans in individuals seropositive and seronegative for HIV-1.
Lancet 1993;341:271-3.
21. Chingbingyong MI, Hughes CV. Detection of Mycoplasma fermentans in human
saliva with a polymerase chain reaction-based assay. Archs Oral Biol
1996;41:311-4.
22. Lo SC, Dawson MS, Newton III PB, Sonoda MA, Shih JW, Engler WF, et al.
Association of the virus-like infectious agent originally reported in patients
with AIDS with acute fatal disease in previously healthy non-AIDS patients.
Amer J Trop Med Hyg 1989;41:364-76.
23. Tully JG, Taylor-Robinson D, Cole RM, Rose DL. A newly discovered
mycoplasma in the human urogenital tract. Lancet 1981;i:1288-91.
24. Tully JG, Taylor-Robinson D, Rose DL, Furr PM, Graham CE, Barile MF.
Urogenital challenge of primate species with Mycoplasma genitalium and
characteristics of infection induced in chimpanzees. J Infect Dis 1986;153:1046-54.
25. Dallo SF, Chavoya A, Su CJ, Baseman JB. DNA and protein sequence homologies
detected between the adhesins of Mycoplasma genitalium and Mycoplasma
pneumoniae. Infect Immun 1989;57:1059-65.
26. Palmer HM, Gilroy CB, Thomas BJ, Naidoo ROM, Taylor-Robinson D. Development
and evaluation of the polymerase chain reaction to detect Mycoplasma
genitalium. FEMS Microbiol Lett 1991;77:199-204.
27. Horner PJ, Gilroy CB, Thomas BJ, Naidoo ROM, Taylor-Robinson D. Association
of Mycoplasma genitalium with acute non-gonococcal urethritis. Lancet 1993;342:582-5.
28. Deguichi T, Komeda H, Yasuda M, Tada K, Iwata H, Asano M, et al. Mycoplasma
genitalium in non-gonococcal urethritis. Int J STD & AIDS 1995;6:144-6.
29. Jensen SJ, Hansen HT, Lind K. Isolation of Mycoplasma genitalium strains
from the male urethra. J Clin Microbiol 1996;34:286-91.
30. Taylor-Robinson D. The history and role of Mycoplasma genitalium in
sexually transmitted diseases. Genitourin Med 1995;71:1-8.
31. Baseman JB, Dallo SF, Tully JG, Rose DL. Isolation and characterization of
Mycoplasma genitalium strains from the human respiratory tract. J Clin
Microbiol 1988;26:2266-9.
32. De Barbeyrac B, Bernet-Poggi C, Febrer F, Renaudin H, Dupon M, Bebear C.
Detection of Mycoplasma pneumoniae and Mycoplasma genitalium in clinical
samples by polymerase chain reaction. Clin Infect Dis 1993;17(Supp1):S83-9.
33. Tully JG, Rose DL, Baseman JB, Dallo SF, Lazzell AL, Davis CP. Mycoplasma
pneumoniae and Mycoplasma genitalium mixture in synovial fluid isolate. J Clin
Microbiol 1995;33:1851-5.
34. Taylor-Robinson D, Gilroy CB, Horowitz S, Horowitz J. Mycoplasma genitalium
in the joints of two patients with arthritis. Eur J Clin Microbiol Infect Dis
1994;13:1066-9.
35. Furr PM, Taylor-Robinson D, Webster ADB. Mycoplasmas and ureaplasmas in
patients with hypogammaglobulinemia and their role in arthritis:
microbiological observations over twenty years. Ann Rheum Dis 1994;53:183-7.
36. Gelfand EW. Unique susceptibility of patients with antibody deficiency to
Mycoplasma infection. Clin Infect Dis 1993;17:S250-3.
37. Mokhbat JE, Person PK, Sabath LD, Robertson JA. Peritonitis due to
Mycoplasma hominis in a renal transplant patient. J Infect Dis 1982;146:713.
38. Burdge DR, Reid GD, Reeve CE, Robertson JA, Stemke GW, Bowie WR. Septic
arthritis due to dual infection with Mycoplasma hominis and Ureaplasma
urealyticum. J Rheumatol 1988;15:366-8.
39. Luttrell LM, Kanj SS, Corey GR, Lins RE, Spinner RJ, Mallon WJ, et al.
Mycoplasma hominis septic arthritis: two case reports and review. Clin Infect
Dis 1994;19:1067-70.
40. Gass R, Fisher J, Badesch D, Zamora M, Weinberg A, Melsness H, et al.
Donor-to-host transmission of Mycoplasma hominis in lung allograft recipients.
Clin Infect Dis 1996;22:567-8.
41. Bonilla HF, Chenoweth CE, Tully JG, Blythe LK, Robertson J, Ognenovski VM,
et al. Mycoplasma felis septic arthritis in a patient with
hypogammaglobulinemia. Clin Infect Dis. In press.
42. Yechouron A, Lefebre J, Robson HG, Rose DL, Tully JG. Fatal septicemia due
to Mycoplasma arginini: a new human zoonosis. Clin Infect Dis 1992;15:434-8.
43. Baseman JB. The cytadhesins of Mycoplasma pneumoniae and M. genitalium. In:
Rottem S, Kahane I, editors. Subcellular biochemistry. New York: Plenum Press,
1993;243-59.
44. Kirchhoff H, Rosegarten R, Lotz W, Fischer M, Lopatta D. Flask-shaped
mycoplasmas: properties and pathogenicity for man and animals. Isr J Med Sci
1984;10:848-53.
45. Gobel U, Speth V, Bredt W. Filamentous structures in adherent Mycoplasma
pneumoniae cells treated with nonionic detergents. J Cell Biol 1981;91:537-43.
46. Krause DC. Mycoplasma pneumoniae cytadherence: unravelling the tie that
binds. Mol Microbiol 1996;20:247-53.
47. Su CJ, Tryon VV, Baseman JB. Cloning and sequence analysis of cytadhesin
gene (P1) from Mycoplasma pneumoniae. Infect Immun 1987;55:3023-9.
48. Dallo SF, Chavoya A, Baseman JB. Characterization of the gene for a
30-kilodalton adhesin-related protein of Mycoplasma pneumoniae. Infect Immun
1990;58:4163-5.
49. Hu PC, Schaper U, Collier AM, Clyde WA, Horikawa M, Huang YS, et al. A
Mycoplasma genitalium protein resembling the Mycoplasma pneumoniae attachment
protein. Infect Immun 1987;55:1126-31.
50. Reddy SP, Rasmussen WG, Baseman JB. Molecular cloning and characterization
of an adherence-related operon of Mycoplasma genitalium. J Bacteriol
1995;177:5943-51.
51. Inamine JM, Loechel S, Gilbert AM, Barile MF, Hu PC. Nucleotide sequence of
the MgPa (mgp) operon of Mycoplasma genitalium and comparison to the P1 (mpp)
operon of Mycoplasma pneumoniae. Gene 1989;82:259-67.
52. Goulet M, Dular R, Tully JG, Billowes G, Kasatiya S. Isolation of
Mycoplasma pneumoniae from the human urogenital tract. J Clin Microbiol
1995;33:2823-5.
53. Reddy SP, Rasmussen WG, Baseman, JB. Isolation and characterization of
transposon Tn 4001-generated, cytadherence-deficient transformants of
Mycoplasma pneumoniae and Mycoplasma genitalium. FEMS Immunol Med Microbiol
1996;15:199-211.
54. Su CJ, Chavoya A, Baseman JB. Regions of Mycoplasma pneumoniae cytadhesin
P1 structural gene exist as multiple copies. Infect Immun 1988;56:3157-61.
55. Dallo SF, Baseman JB. Adhesin gene of Mycoplasma genitalium exists as
multiple copies. Microb Pathog 1991;10:475-80.
56. Peterson SN, Bailey CC, Jensen JS, Borre MB, King ES, Bott KF, et al.
Characterization of repetitive DNA in the Mycoplasma genitalium genome:
possible role in the generation of antigenic variation. Proc Natl Acad Sci USA
1995;92:11829-33.
57. Dallo SF, Horton JR, Su CJ, Baseman JB. Restriction fragment length
polymorphism in the cytadhesin P1 gene of human clinical isolates of Mycoplasma
pneumoniae. Infect
Immun 1990;58:2017-20.
58. Su CJ, Chavoya A, Dallo SF, Baseman JB. Sequence divergency of the cytadhesin
gene of Mycoplasma pneumoniae. Infect Immun 1990;58:2669-74.
59. Su CJ, Dallo SF, Baseman JB. Possible origin of sequence divergence in the
P1 cytadhesin gene of Mycoplasma pneumoniae. Infect Immun 1993;61:816-22.
60. Dallo SF, Su CJ, Horton JR, Baseman JB. Identification of P1 gene domain
containing epitope(s) mediating Mycoplasma pneumoniae cytadherence. J Exp Med
1988;167:718-23.
61. Gerstenecker B, Jacobs E. Topographical mapping of the P1-adhesin of
Mycoplasma pneumoniae with adherence-inhibiting monoclonal antibodies. J Gen
Microbiol 1990;136:471-6.
62. Dallo SF, Lazzell AL, Chavoya A, Reddy SP, Baseman JB. Biofunctional
domains of the Mycoplasma pneumoniae P30 adhesin. Infect Immun
1996;64:2595-601.
63. Layh-Schmitt G, Hilbert H, Pirkl E. A spontaneous hemadsorption-negative
mutant of Mycoplasma pneumoniae exhibits a truncated adhesin-related
30-kilodalton protein and lacks the cytadherence-accessory protein HMW1. J
Bacteriol 1995;177:843-6.
64. Reddy SP, Rasmussen WG, Baseman JB. Correlations between Mycoplasma
pneumoniae sensitivity to cyclosporin A and cyclophilin-mediated regulation of
mycoplasma cytadherence. Microb Pathog 1995;20:155-69.
65. Biberfeld G. Infection sequelae and autoimmune reactions in Mycoplasma
pneumoniae infection. In: Razin S, Barile MF, editors. The Mycoplasmas Vol. IV.
New York: Academic Press, 1985:293-311.
66. Cunningham MW. Molecular mimicry: bacterial antigen mimicry. In: Bona CA,
Siminovitch K, Theofilopoulos AN, Zanetti M, editors. The pathology of
autoimmunity. New York: Harwood Academic Publishers, 1993:245-56.
67. Bisset LR. The Mycoplasma genitalium adhesin protein and several human
class II MHC proteins exhibit sequence homology: possible ramifications for the
development of autoimmunity. Autoimmunity 1992;14:167-8.
68. Root-Bernstein RS, Hobbs SH. Homologies between mycoplasma adhesion
peptide, CD4 and class II MHC proteins: a possible mechanism for HIV-mycoplasma
synergism in AIDS. Res Immunol 1991;142:519-23.
69. Cole BC. Mycoplasma interactions with the immune system: implications for
disease pathology. ASM News 1996;62:471-5.
70. Rawadi G, Roman-Roman S. Mycoplasma membrane lipoproteins induce
proinflammatory cytokines by a mechanism distinct from that of lipopolysaccharide.
Infect Immun 1996;64:637-43.
71. Theiss P, Karpas A, Wise KS. Antigenic topology of the P29 surface
lipoprotein of Mycoplasma fermentans: differential display of epitopes results
in high-frequency phase variation. Infect Immun 1996;64:1800-9.
72. Baseman JB, Lange M, Criscimagna NL, Girón JA, Thomas CA. Interplay between
mycoplasmas and host target cells. Microb Pathog 1995;19:105-16.
73. Girón JA, Lange M, Baseman JB. Adherence, fibronectin binding, and
induction of cytoskeleton reorganization in cultured human cells by Mycoplasma
penetrans. Infect Immun 1996;64:197-208.
74. Blanchard A, Montagnier L. AIDS-associated mycoplasmas. Annu Rev Microbiol
1994;48:687-712.
75. Wang RY-H, Shih J W-K, Weiss SH, Grandinetti T, Pierce PF, Lange M, et al.
Mycoplasma penetrans infection in male homosexuals with AIDS: high
seroprevalence and association with Kaposi's Sarcoma. Clin Infect
Dis1993;17:724-9.
76. Grau O, Slizewicz B, Tuppin P, Launay V, Bourgeois E, Sagot N, et al.
Association of Mycoplasma penetrans with human immunodeficiency virus
infection. J Infect Dis1995;172:672-81.
77. Paton GR, Jacobs JP, Perkins FT. Chromosome changes in human diploid-cell
cultures infected with Mycoplasma. Nature 1966;207:43-5.
78. Macpherson I, Russell W. Transformations in hamster cells mediated by
mycoplasmas. Nature 1966;210:1343-5.
79. Kangro HO, Chong SKF, Hardiman A, Heath RB, Walker-Smith JA. A prospective
study of viral and mycoplasma infections in chronic inflammatory bowel disease.
Gastroenterology 1990;98:549-53.
Emerging Infectious Diseases National Center for Infectious Diseases Centers
for Disease Control and Prevention Atlanta, GA