The story of Kaitlin Hunter [1] brings to light the potential triumphs of the age
of biotechnology and how an understanding of the interplay of genomics and the human
microbiome can provide a cure to a life-threatening disease. After a serious car accident
and under standard healthcare, Kaitlin was given antibiotics to prevent infection.
Likely, the antibiotic treatment compromised her normal gastrointestinal flora and
permitted Clostridium difficile, a toxin-producing, Gram-positive, anaerobic, spore-forming
bacillus, to become established. C. difficile causes diarrhea and is linked to approximately
14,000 deaths each year in the United States alone [2]. However, a novel solution
was undertaken to treat Kaitlin - her mother, a healthy donor, provided a fecal sample
which was transplanted into Kaitlin’s colon. Her mother’s bacteria re-colonized the
colon and Kaitlin was cured. This life-saving treatment may make one reconsider the
phrase of ‘taking no “_ _ _ _” from anyone’.
While a fecal transplant makes logical sense for staving off a C. difficile infection,
there are patients (and physicians) who may not opt for such a treatment. First, patients
may not relish the thought of receiving fecal matter that would be infused directly
into their colons. The thought of it is unpleasant at best. Second, a fecal sample
even from a healthy donor would be replete with bacteria, some of which may be pathogenic
or at least opportunistic pathogens. However, Petrof et al. [3] have devised a solution
to ‘RePOOPulate’ the intestines of patients with C. difficile infections. They used
investigative genetics technology to develop a stool substitute, which poses less
risk to the patient, and probably for the first time employed massively parallel sequencing
(MPS) to track a transplant and monitor a patient’s recovery. Thereby, they demonstrated
that the disruptive MPS technology has immediate diagnostic applications.
Petrof et al. obtained a stool sample from a healthy, 41-year-old woman and isolated
62 different bacteria. After rejecting antibiotic-resistant microbes - those that
may cause disease, 33 intestinal bacteria isolates remained. These isolates were reconstituted
in proportions to approximate those from the original stool sample. Thus Petrof at
el. created a stool substitute mixture comprised of a multispecies community no longer
in the presence of fecal material.
Two patients were selected for ‘repoopulation’. They were a 74-year-old Caucasian
woman with six episodes of recurrent C. difficile infection over an 18-month period
and a 70-year-old Caucasian woman with a history of peripheral neuropathy, which predisposed
her to recurrent skin and soft tissue infections and under cefazolin treatment developed
a C. difficile infection. Both were infected with a particularly hypervirulent strain
of C. difficile, ribotype 078. These patients posed a challenge because of age and
recurrent infection.
The status of pretreatment and post-treatment microbiota was monitored by sequencing
PCR products of the bacterial V6 rRNA region on the Ion Torrent platform with low
to medium throughput chips for the instrument. The Ion Torrent is one of the commercially
available massively parallel sequencers that enables genomic analyses on the bench
top of most laboratories which was only a short time ago the domain of large genomic
centers. Throughput of the sequencing chips is upwards of 100 megabases and for single
patient monitoring was deemed sufficient to obtain a depth of coverage to assess diversity
of the patients’ intestinal microbial flora. Up to 12 samples were multiplexed on
each chip through use of indexing. Therefore community microbial composition analysis
could be assessed in virtually real-time (that is, 24 to 48 h) to track the success
or failure of the stool substitute transplant to re-establish the microbiota of the
patients.
Sufficient V6 rRNA reads were obtained (between 3,758 and 76,752 V6 rRNA reads per
sample for Patient 1 and between 19,751 and 64,200 reads per sample for Patient 2)
to estimate general and relative diversity of the microflora of the patients. Within
2 to 3 days of stool substitute treatment, each patient recovered a normal bowel pattern
and remained symptom-free for up to 6 months when monitoring was stopped. The first
patient displayed a highly diverse microbiota that after treatment became less diverse
and after 6 months regained similar diversity as that of pretreatment. The second
patient’s microbiota had relatively low diversity and became more diverse following
treatment which stabilized with a higher diversity than that of pretreatment. Genomic
analyses demonstrated that the rRNA sequences representative of the stool substitute
were infrequent in the pretreatment stool samples of the patients. Once stabilized,
the same sequences comprised >25% of the patients’ samples.
Taxonomic assignment with rRNA V6 region could only be carried out at the family level
as greater phylogenetic resolution cannot be attained using a single house-keeping
gene. This lack of resolution did not compromise monitoring for stool substitute transplantation
success. However, given the throughput of MPS, adding a few more housekeeping genes
could easily provide species/strain level resolution and even monitor for mutation
that may arise.
Although successful, the RePOOPulation study was limited to two patients and more
studies are needed. However, Petrof et al. have demonstrated the proof of concept
that this stool substitute, synthetically reconstituted from fecal material, can be
an effective treatment for C. difficile infection, particularly for recurrent infections
with hypervirulent strains. The authors point out that there are several advantages
to using a substitute over actual fecal material, besides the obvious distaste of
having such material injected into one’s body. These include ‘the exact composition
of bacteria administered is known and can be controlled; the bacterial species composition
can be reproduced, should a future treatment be necessary; preparations of pure culture
are more stable than stool, which some groups recommend should be collected fresh
and instilled into the recipient within 6 h of collection; an absence of viruses and
other pathogens in the administered mixture can be ensured, thereby improving patient
safety; and the administered organisms can be selected based on their sensitivity
to antimicrobials, allowing an enhanced safety profile’.
It is hard to believe that only a few years ago the human microbiome was defined solely
by E. coli and bacteria that caused bad breath and tooth decay. The diversity of the
human microbiome is substantial and its secrets, as they unravel, promise to bring
additional insights to human health and potential treatments to improve well-being.
Investigative genetics tools, such as high throughput sequencing and targeted gene
diagnostics, will figure prominently into our personalized medical treatment and fecal,
or simulate, transplantation is just the tip of the iceberg. Who knows… the next time
one of us travels to an area of the world where the microflora of the water can cause
intestinal discomfort, a possible pretreatment for better well-being during travel
may be a stool simulant enema.
Competing interests
This author has no competing interests.