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The Hospital Microbiome Project:
        Experimental Designs for Investigating the
        Development of Microbial Communities


Daniel Patrick Smith

Hospital Microbiome Workshop
University of Chicago, 6.7.2012
Background

How microbial communities
persist and change in indoor
environments is of immense
interest to public health
bodies and scientists.

     Demographics of a building
      play a key role in shaping
      microbial communities.
        – Humans aerosolize up to 37
          million bacteria per person-
          hour (Qian, 2012)
        – Forensic microbiology can
          determine who last touched
          an object by their
          microbiota. (Fierer, 2010)

    Qian, J., Hospodsky, D., Yamamoto, N., Nazaroff, W. W. & Peccia, J. Indoor Air (2012).
    Fisk, W. J. Annual Review of Energy and the Environment 25, 537–566 (2000).
    Fierer, N. et al. Proceedings of the National Academy of Sciences 107, 6477–6481 (2010).
Background:
Hospitals as a Sampling Site
A newly constructed hospital
presents the ideal conditions for
studying the development of
bacterial communities driven by
human demographics.
     – Patient rooms are identically
       constructed – replicates.
     – Building materials are defined.
     – Closed environment.
     – No prior pathogenic contamination.
     – Relevant microorganisms are
       thoroughly characterized.


 Hospital Microbiome Workshop
Background:
Hospital Acquired Infections (HAI)

 The ten most common pathogens:
     –   coagulase-negative staphylococci
     –   Staphylococcus aureus
     –   Enterococcus species
     –   Candida species
     –   Escherichia coli                                                  Accounted for 84% of
     –   Pseudomonas aeruginosa                                            the observed HAIs in
     –   Klebsiella pneumoniae                                             463 hospitals over a
     –   Enterobacter species                                              21 month period.
     –   Acinetobacter baumannii                                           (Hidron, 2008)
     –   Klebsiella oxytoca


 Hidron, A. I. et al. Infection Control and Hospital Epidemiology 29, 996–1011 (2008).
Background:
 Hospital vs. Non-Hospital Infections
                           Contracted        Fatal (% Fatal)
       Hospital            1.7 million       99,000 (6%)
       Non-Hospital        1.5 million       15,743 (1%)
                                            Cause of Death – Total over U.S. in 2002                Number
                                      1.    Diseases of heart                                       696,947
                                      2.    Malignant neoplasms                                     557,271
4.5 Infections per                    3.    Cerebrovascular diseases                                162,672
100 Hospital admissions               4.    Chronic lower respiratory diseases                      124,816
                                      5.    Accidents (unintentional injuries)                      106,742
                                            Hospital Acquired Infection - associated                99,000
                                      6.    Diabetes mellitus                                       73,249
                                      7.    Influenza and pneumonia                                 65,681
                                      8.    Alzheimer’s disease                                     58,866

   Groseclose SL, et al. (2004) MMWR Morb Mortal Wkly Rep 51: 1–84.    Anderson RN, Smith BL (2005) Natl Vital Stat Rep 53: 1–89.
   Hall-Baker PA, et al. (2010) MMWR Morb Mortal Wkly Rep 57: 1–100.   Klevens RM, et al. (2007) Public Health Rep 122: 160–166.
Project Goal
 Determine which environmental parameters have the
  greatest influence on the development of microbial
  communities within a hospital.
           – Patient/Staff Microflora   – Light Level/Source
           – Building Material          – Demographic Exposure
           – Temperature/Humidity          • High vs Low Traffic
                                           • Staff vs Patient Area

 Understand how demographics interact with the
  succession of microorganisms in a hospital.




 Hospital Microbiome Workshop
Guiding Hypotheses
1.       Microbial community structure on hospital surfaces can be predicted by
         human demographics, physical conditions (e.g. humidity, temperature),
         and building materials for each location and time.

2.       A patient-room microbiota is influenced by the current patient and
         their duration of occupancy, and shows community succession with the
         introduction of a new occupant.

3.       The colonization of the surfaces and patients by potential pathogens is
         influenced by composition and diversity of the existing microbial
         community derived from previous occupants of the space.

4.       The rate of microbial succession is driven by demographic usage and
         building materials.



     Hospital Microbiome Workshop
Ideal Sampling Strategy:
Daily Sampling of Bacterial Reservoirs for a Year.

Patient Area                         Water                             Travel Areas
Bed rails, tray table, call boxes,   Cold tap water, hot tap water,    Corridor floor & wall, stairwell
telephone, bedside tables,           water used to clean floors.       handrail & steps & door knobs
patient chair, IV pole, floor,                                         & kick plates, elevator buttons
light switches, air exhaust.         Patient                           & floor & handrail.
                                     Stool sample, nasal swab, hand.
Patient Restroom                                                       Lobby
Sink, light switches, door knob,     Staff                             Front desk surface, chairs,
handrails, toilet seats, flush                                         coffee tables, floor.
lever, bed pan cleaning              Nasal swab, bottom of shoe,
equipment, floor.                    dominant hand, cell phone,
                                     computer mouse, work phone,       Public Restroom
                                     shirt cuff, stethoscope.          Floor, door handles, sink
Additional Equipment                                                   controls, sink bowl, soap
IV Pump control panel, monitor 240 Patient Rooms + 50 Staff            dispenser, towel dispenser,
control panel, monitor touch   = 2,437,105 samples                     toilet seats, toilet lever, stall
screen, monitor cables,        = $24 million in extraction &           door lock, stall door handle,
ventilator control panel.      sequencing consumables alone            urinal flush lever.
  Hospital Microbiome Workshop
Reduced Sampling Strategy:
Weekly Sampling for a Year of 187 Sites

Human                            Patient Room (x20)     Nurse Station (x1)
 Patients (≤ 20)                 Floor                 Countertop
     – Nose                       Bedrail               Computer mouse
     – Stool                      IV control panel      Phone handle
 Staff (x5)                      Faucet handle         Chair
     –    Nose                    Outer door handle     Corridor floor
     –    Uniform cuff
                                  Air exhaust filter    Hot tap water
     –    Pen
                                                         Cold tap water
     –    Cell phone




  Hospital Microbiome Workshop
Sampling Airborne Microorganisms

 Each patient room has independent exhaust vents which can
  be fitted with removable filters for this study.
     – Replace filters weekly.
     – Use ventilation rate, filter efficiency, and microbial abundance to
       calculate the concentration of airborne microorganisms.


  Further interrogation via particle
   deposition onto blood-agar plates
   for a 1 hr period, followed by
   challenging of colonies with
   antibiotic susceptibility tests.


 Hospital Microbiome Workshop
Sampling Protocol:
Compatible with Quantitative Analyses

 Sterile swabs moistened with saline solution will be used to
  sample a region of pre-defined dimensions.
     – qRT-PCR provides an estimate of genomes, yielding cells/cm2
     – Allows conclusions to be drawn regarding actual abundance of
       microbial taxa, rather than relative abundance.

  Hot and cold water supplies
        – Single location
        – Run for 15 sec
        – Extract from 100 uL




 Hospital Microbiome Workshop
Sample Selection

 Although 20 patient rooms and their occupants will be
  sampled, only 8 will be selected for sequencing.
     – Dramatically reduces expenses for sample prep & sequencing.
     – 4 rooms in which HAIs were contracted.
     – 4 rooms in which HAIs were NOT contracted.


 Addresses the hypothesis:
     The colonization of the surfaces and patients by potential pathogens is
     influenced by composition and diversity of the existing microbial
     community derived from previous occupants of the space.



 Hospital Microbiome Workshop
Passive Monitoring

 Data loggers will be placed in patient
  rooms to take hourly measurements of:
     – Temperature
     – Relative Humidity
     – Dew Point


 National Oceanic and Atmospheric
  Administration records will be used to
  obtain data on outdoor environmental
  conditions.


 Hospital Microbiome Workshop
Patient Infections

 We will request IRB approval for accessing pathogen reports
  for patients participating in this study if they contract, or are
  admitted with, an infection.




 Hospital Microbiome Workshop
Project Timeline

 November 2012
     – Conduct survey of building materials.
     – Identify all sampling locations in the building, and begin collecting
       surface, air, and water samples.
     – Secure and activate data loggers in patient rooms.
 December 2012
     – Identify staff members who wish to participate and begin sampling
       them in their current working environment.
 January 31st, 2013 – Hospital Opens
     – Identify patients who wish to participate and begin sampling them a
       they are admitted to the rooms under obervation.


 Hospital Microbiome Workshop
Sample Processing

 Swab tips are cut off and placed in a lysis/PCR solution.
 After incubation and thorough mixing, aliquots are
  distributed to 96-well PCR plates in triplicate.
 Amplification of 16S/18S/ITS takes place in a qualitative real
  time (qRT) PCR machine using barcoded primers.
 Samples are pooled into groups of 500 and sequenced to a
  depth of 3,000 read pairs (2 x 150 bp) per sample.
 Reads are filtered for quality, merged into 250 bp reads, and
  demultiplexed based on barcode.


 Hospital Microbiome Workshop
Data Analysis

 The QIIME software suite will be used to:
     –   Cluster reads into operational taxonomic units (OTUs).
     –   Phylogenetically classify OTUs based on reference databases.
     –   Calculate alpha and beta diversity among samples.
     –   Visualize sample similarity via principle coordinate analysis plots.




 Caporaso, J. G. et al. Nature Methods 7, 335-336 (2010).
Data Analysis

 SourceTracker will be used to:
     – Identify sources and proportions of contamination on surfaces.
     – Answer questions such as “What proportion of the air’s microbes
       originate from a patient’s nasal microbiome?”




 Knights, D. et al. Nature Methods 8, 761-763 (2011).
Data Analysis

 Microbial Assemblage Prediction (MAP) will be used to:
     – Predict the relative abundance of microorganisms in an
       environment, given set of environmental conditions.
     – Simulate how community composition will shift if an environmental
       variable is altered.

              Env. Parameter
              Rhodobacteriales
              Flavobacteriales
              Rickettsiales
              Pseudomonadales
              Opitutales
              Vibrionales
              Rhizobiales




 Larsen, P. E., Field, D. & Gilbert, J. A. Nature Methods (2012).
Data Analysis
 Local Similarity Analysis will be used to:
     – Identify patterns in microbial succession. E.g. if organism A is
       blooming now, then organism B will bloom in a few weeks.




 Gilbert, J. A. et al. The ISME Journal 6, 298-308 (2011).
Project Scope
 We are currently pursing a grant that will enable processing
  of 4,732 samples collected over 52 weeks from 91 locations:
   Human                        Patient Room (x8)       Nurse Station (x1)
    Patients (≤ 8)              Floor                  Countertop
            – Nose               Bedrail                Computer mouse
            – Stool              IV control panel       Phone handle
         Staff (x5)             Faucet handle          Chair
            –    Nose            Outer door handle      Corridor floor
            –    Uniform cuff
                                 Air exhaust filter     Hot tap water
            –    Pen
            –    Cell phone                              Cold tap water

 Additional funding could allow for:
       – More frequent collection              – Increased replication
       – Additional sampling locations         – Introduction of variables
       – Longer time-course                        • Cancer vs. surgery wards
                                                   • North vs. south facing windows
 Hospital Microbiome Workshop

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Hospital Microbiome Project Proposal

  • 1. The Hospital Microbiome Project: Experimental Designs for Investigating the Development of Microbial Communities Daniel Patrick Smith Hospital Microbiome Workshop University of Chicago, 6.7.2012
  • 2. Background How microbial communities persist and change in indoor environments is of immense interest to public health bodies and scientists.  Demographics of a building play a key role in shaping microbial communities. – Humans aerosolize up to 37 million bacteria per person- hour (Qian, 2012) – Forensic microbiology can determine who last touched an object by their microbiota. (Fierer, 2010) Qian, J., Hospodsky, D., Yamamoto, N., Nazaroff, W. W. & Peccia, J. Indoor Air (2012). Fisk, W. J. Annual Review of Energy and the Environment 25, 537–566 (2000). Fierer, N. et al. Proceedings of the National Academy of Sciences 107, 6477–6481 (2010).
  • 3. Background: Hospitals as a Sampling Site A newly constructed hospital presents the ideal conditions for studying the development of bacterial communities driven by human demographics. – Patient rooms are identically constructed – replicates. – Building materials are defined. – Closed environment. – No prior pathogenic contamination. – Relevant microorganisms are thoroughly characterized. Hospital Microbiome Workshop
  • 4. Background: Hospital Acquired Infections (HAI)  The ten most common pathogens: – coagulase-negative staphylococci – Staphylococcus aureus – Enterococcus species – Candida species – Escherichia coli Accounted for 84% of – Pseudomonas aeruginosa the observed HAIs in – Klebsiella pneumoniae 463 hospitals over a – Enterobacter species 21 month period. – Acinetobacter baumannii (Hidron, 2008) – Klebsiella oxytoca Hidron, A. I. et al. Infection Control and Hospital Epidemiology 29, 996–1011 (2008).
  • 5. Background: Hospital vs. Non-Hospital Infections Contracted Fatal (% Fatal) Hospital 1.7 million 99,000 (6%) Non-Hospital 1.5 million 15,743 (1%) Cause of Death – Total over U.S. in 2002 Number 1. Diseases of heart 696,947 2. Malignant neoplasms 557,271 4.5 Infections per 3. Cerebrovascular diseases 162,672 100 Hospital admissions 4. Chronic lower respiratory diseases 124,816 5. Accidents (unintentional injuries) 106,742 Hospital Acquired Infection - associated 99,000 6. Diabetes mellitus 73,249 7. Influenza and pneumonia 65,681 8. Alzheimer’s disease 58,866 Groseclose SL, et al. (2004) MMWR Morb Mortal Wkly Rep 51: 1–84. Anderson RN, Smith BL (2005) Natl Vital Stat Rep 53: 1–89. Hall-Baker PA, et al. (2010) MMWR Morb Mortal Wkly Rep 57: 1–100. Klevens RM, et al. (2007) Public Health Rep 122: 160–166.
  • 6. Project Goal  Determine which environmental parameters have the greatest influence on the development of microbial communities within a hospital. – Patient/Staff Microflora – Light Level/Source – Building Material – Demographic Exposure – Temperature/Humidity • High vs Low Traffic • Staff vs Patient Area  Understand how demographics interact with the succession of microorganisms in a hospital. Hospital Microbiome Workshop
  • 7. Guiding Hypotheses 1. Microbial community structure on hospital surfaces can be predicted by human demographics, physical conditions (e.g. humidity, temperature), and building materials for each location and time. 2. A patient-room microbiota is influenced by the current patient and their duration of occupancy, and shows community succession with the introduction of a new occupant. 3. The colonization of the surfaces and patients by potential pathogens is influenced by composition and diversity of the existing microbial community derived from previous occupants of the space. 4. The rate of microbial succession is driven by demographic usage and building materials. Hospital Microbiome Workshop
  • 8. Ideal Sampling Strategy: Daily Sampling of Bacterial Reservoirs for a Year. Patient Area Water Travel Areas Bed rails, tray table, call boxes, Cold tap water, hot tap water, Corridor floor & wall, stairwell telephone, bedside tables, water used to clean floors. handrail & steps & door knobs patient chair, IV pole, floor, & kick plates, elevator buttons light switches, air exhaust. Patient & floor & handrail. Stool sample, nasal swab, hand. Patient Restroom Lobby Sink, light switches, door knob, Staff Front desk surface, chairs, handrails, toilet seats, flush coffee tables, floor. lever, bed pan cleaning Nasal swab, bottom of shoe, equipment, floor. dominant hand, cell phone, computer mouse, work phone, Public Restroom shirt cuff, stethoscope. Floor, door handles, sink Additional Equipment controls, sink bowl, soap IV Pump control panel, monitor 240 Patient Rooms + 50 Staff dispenser, towel dispenser, control panel, monitor touch = 2,437,105 samples toilet seats, toilet lever, stall screen, monitor cables, = $24 million in extraction & door lock, stall door handle, ventilator control panel. sequencing consumables alone urinal flush lever. Hospital Microbiome Workshop
  • 9. Reduced Sampling Strategy: Weekly Sampling for a Year of 187 Sites Human Patient Room (x20) Nurse Station (x1)  Patients (≤ 20)  Floor  Countertop – Nose  Bedrail  Computer mouse – Stool  IV control panel  Phone handle  Staff (x5)  Faucet handle  Chair – Nose  Outer door handle  Corridor floor – Uniform cuff  Air exhaust filter  Hot tap water – Pen  Cold tap water – Cell phone Hospital Microbiome Workshop
  • 10. Sampling Airborne Microorganisms  Each patient room has independent exhaust vents which can be fitted with removable filters for this study. – Replace filters weekly. – Use ventilation rate, filter efficiency, and microbial abundance to calculate the concentration of airborne microorganisms.  Further interrogation via particle deposition onto blood-agar plates for a 1 hr period, followed by challenging of colonies with antibiotic susceptibility tests. Hospital Microbiome Workshop
  • 11. Sampling Protocol: Compatible with Quantitative Analyses  Sterile swabs moistened with saline solution will be used to sample a region of pre-defined dimensions. – qRT-PCR provides an estimate of genomes, yielding cells/cm2 – Allows conclusions to be drawn regarding actual abundance of microbial taxa, rather than relative abundance.  Hot and cold water supplies – Single location – Run for 15 sec – Extract from 100 uL Hospital Microbiome Workshop
  • 12. Sample Selection  Although 20 patient rooms and their occupants will be sampled, only 8 will be selected for sequencing. – Dramatically reduces expenses for sample prep & sequencing. – 4 rooms in which HAIs were contracted. – 4 rooms in which HAIs were NOT contracted.  Addresses the hypothesis: The colonization of the surfaces and patients by potential pathogens is influenced by composition and diversity of the existing microbial community derived from previous occupants of the space. Hospital Microbiome Workshop
  • 13. Passive Monitoring  Data loggers will be placed in patient rooms to take hourly measurements of: – Temperature – Relative Humidity – Dew Point  National Oceanic and Atmospheric Administration records will be used to obtain data on outdoor environmental conditions. Hospital Microbiome Workshop
  • 14. Patient Infections  We will request IRB approval for accessing pathogen reports for patients participating in this study if they contract, or are admitted with, an infection. Hospital Microbiome Workshop
  • 15. Project Timeline  November 2012 – Conduct survey of building materials. – Identify all sampling locations in the building, and begin collecting surface, air, and water samples. – Secure and activate data loggers in patient rooms.  December 2012 – Identify staff members who wish to participate and begin sampling them in their current working environment.  January 31st, 2013 – Hospital Opens – Identify patients who wish to participate and begin sampling them a they are admitted to the rooms under obervation. Hospital Microbiome Workshop
  • 16. Sample Processing  Swab tips are cut off and placed in a lysis/PCR solution.  After incubation and thorough mixing, aliquots are distributed to 96-well PCR plates in triplicate.  Amplification of 16S/18S/ITS takes place in a qualitative real time (qRT) PCR machine using barcoded primers.  Samples are pooled into groups of 500 and sequenced to a depth of 3,000 read pairs (2 x 150 bp) per sample.  Reads are filtered for quality, merged into 250 bp reads, and demultiplexed based on barcode. Hospital Microbiome Workshop
  • 17. Data Analysis  The QIIME software suite will be used to: – Cluster reads into operational taxonomic units (OTUs). – Phylogenetically classify OTUs based on reference databases. – Calculate alpha and beta diversity among samples. – Visualize sample similarity via principle coordinate analysis plots. Caporaso, J. G. et al. Nature Methods 7, 335-336 (2010).
  • 18. Data Analysis  SourceTracker will be used to: – Identify sources and proportions of contamination on surfaces. – Answer questions such as “What proportion of the air’s microbes originate from a patient’s nasal microbiome?” Knights, D. et al. Nature Methods 8, 761-763 (2011).
  • 19. Data Analysis  Microbial Assemblage Prediction (MAP) will be used to: – Predict the relative abundance of microorganisms in an environment, given set of environmental conditions. – Simulate how community composition will shift if an environmental variable is altered. Env. Parameter Rhodobacteriales Flavobacteriales Rickettsiales Pseudomonadales Opitutales Vibrionales Rhizobiales Larsen, P. E., Field, D. & Gilbert, J. A. Nature Methods (2012).
  • 20. Data Analysis  Local Similarity Analysis will be used to: – Identify patterns in microbial succession. E.g. if organism A is blooming now, then organism B will bloom in a few weeks. Gilbert, J. A. et al. The ISME Journal 6, 298-308 (2011).
  • 21. Project Scope  We are currently pursing a grant that will enable processing of 4,732 samples collected over 52 weeks from 91 locations: Human Patient Room (x8) Nurse Station (x1)  Patients (≤ 8)  Floor  Countertop – Nose  Bedrail  Computer mouse – Stool  IV control panel  Phone handle  Staff (x5)  Faucet handle  Chair – Nose  Outer door handle  Corridor floor – Uniform cuff  Air exhaust filter  Hot tap water – Pen – Cell phone  Cold tap water  Additional funding could allow for: – More frequent collection – Increased replication – Additional sampling locations – Introduction of variables – Longer time-course • Cancer vs. surgery wards • North vs. south facing windows Hospital Microbiome Workshop