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Design of Bacterial Bioreporters for Their
Application in Assays of Harmful Chemicals in
            Different Environment

           Raghu H V & Kumar N.
Introduction

Physico-chemical analysis

 High selectivity, sensitivity, accuracy and reproducibility

 Drawbacks–

    Limited to predetermined set of substances,

    Fails to indicate bioavailability

    Time consuming, expensive & requires lot of expertise
Bioreporters

• Measures Bioavailable concentration

• Predict the fate & availability

• Cost effective

• Multianalyte approach

• Detects group of compound rather single analyte
What are Bioreporter?
A microorganisms, cell culture or cell line, often genetically engineered,
with an activity that reflects changes in environmental conditions in dose
response dependent manner

                                                                 Signal



                            Transcription    Translation
         Promoter



                    Reporter                m RNA
                                                      Reporter
                     gene
                                                       protein



   Analyte
Principle of Bacterial Bioreporters


 Analyte                Bacterial                  Signal
                      Bioreporters


                   Molecular recognition or
                  Physico-chemical condition




   Class I                Class II                      Class III

    Target                Stress                       Compound
 compound-            Increase in the                   or Stress
Increase in the           out put                      decrease in
    out put                                            the out put

                                               (van der Meer et al., 2004)
Cont…
                                                  Analyte                                          RNA
                                                degraded to                                     polymerase
                                                  effector
                   Periplasmic                                       Regulator
Analyte A            binding                                A
                  protein binds
                     analyte
                                            A
                                                      operator        promoter      Reporter

                            Transport/                      Regulator recruits/ activates
                                          Analyte
      Diffusion             Diffusion                            RAN polymerase
                                          binds to
                                         regulator
                                                            A

                                                       operator        promoter      Reporter

                                                                                                Signal
                                   Reporter protein
                                     synthesized
                                                            A          mRNA                       Reporter
                                                                                                  protein,
                                                                                                  quantum
                                                       operator        promoter      Reporter       yield,
                                         CM                                                       stability,
                                                                                                  specific
                                                  Cytosol
                                                                                                   activity
            out
                                                                       (van der Meer et al., 2004)
Fundamentals of Bioreporter
 Promoter


                                   Transcription       Translation
                                                                                 Lights On

                        Reporter                    m RNA
                         gene                                      Reporter
                                                                    protein


Analyte or
 stress
                                           Transcription                      Lights
                                                   Transcription                off
                              Toxic
                                                     Translation
             Promoter


                            Reporter
                             gene                                     Reporter
                                                   Transcription       protein
                              No                   Translation
                             Toxic
       Analyte                                                          Lights On
                                       (Xu et al., 2012)
Reporter gene
Firefly luciferase (luc)
Bacterial luciferase (lux)
Green fluorescent protein (GFP)
Chloramphenicol acetyltransferase (CAT)
Aequorin
Uroporphyrinogen III methyltransferases
β-galactosidase
β-lactamase
Alkaline phosphatase (SPAP)



                                           (New et al., 2003)
Firefly Luciferase (luc)

 luc gene derived from Photinus pyralis
 High light out and rapid response kinetics
                                 Mg2+
  luciferase + luciferin + ATP           Luciferase. luciferyl-AMP + PPi


Luciferase. luciferyl-AMP + O2          luciferase + oxyluciferin + AMP + C02 + hv


Exogenous addition of luciferin substrate

Not able to react autonomously or monitor

Maximal light output translates into very sensitive assay
Luciferase (lux gene)




                        (Close et al., 2009)
lux Gene
• lux AB genes
   – Encodes only luciferase
   – Exogenous addition of aldehyde (n-dacanol)
   – Brighter & easier signal

• lux CDABE genes
   – Continuous substrate independent signaling
   – Accommodate complete gene cassettes
   – Contains full complement of luciferase-luciferrin complex
   – Real time to near real time capabilities
• lux CDABE operon synthetically optimized away from its
  native AT rich state to towards GC rich MO’s
Green Fluorescent Protein (GFP)

Photoprotein         clone   from   jelly   fish
Aequorea Victoria

Doesn't    require     any   substrate      and
dependent on external light source

Functioning semi-continuously and near
real time

Dual color formats at different spectra
Fluorescent Reporter Protein in Array System


Protein   Excitation   Emission
 GFP         395         509
 EGFP        488         509
 BFP         380         440
GFPuv        395         509
 YFP         513         527
 CFP         433         475
 CobA        357         605
 RFP         558         583
Aequorin
Ca2+ sensitive luminescent protein – Aequorea aequorea




- Inhibited by Mg2+ and also triggered by Eu2+, Sr2+ and Ba2+ Multifaceted
                reporter protein with Affinities (KD) 1-10µL
Chloramphenicol Acetyltransferase
                     (CAT)
                                          CAT gene
    Acetyl coenzyme A + Chloramphenicol              CoA + CAP-3 Acetate



•   Radiolabelled (14 C or 3H) CAP by autoradiography & liquid scintillation
    counting
•   Fluorescent measurement
•   Ex: CAT TOX (L) assay
β-Galactosidase
•   LacZ gene from E.coli encodes a β-Galactosidase enzyme

•   Hydrolysis of β-galactoside disaccharide into monosaccharide yield
    colorimetric signal

•   SOS chromotest – LacZ fusions to DNA to monitor mutagenic/
    Carcinogenic genotoxic compound

•   Luminescent, chemiluminescent or fluorescent endpoint also possible

•   Contribute to elevated background signal

•   Delayed data accumulation
Uroporphyrinogen (Urogen) III
                Methyltransferases (UMT)
 Important for the biosynthetic pathways of vitamin B12 and siroheme
 Vitamin B12 - cobA genes in Bacillus megatarium, Methanobacterium ivanovii,
  Propionibacterium freudenreichii, and Pseudomonas denitrificans.
 Second form of UMT is encoded by the cysG gene in E. coli and S.
  typhimurium.
 Bioreporter for the selection of recombinant plasmids, as a marker for gene
  transcription, and for the detection of toxic salts such as arsenite and
  antimonite.




                                                                        300 nm

                                                                        Red to
                                                                         red-
                                                                        orange
β-lactamases

•   Cleaves penicillin and cephalosporin

•   TEM-1 β-lactamses (E.coli) engineered into cytosolic membrane
    associated forms

•   Membrane permeable flourogenic substrate CCF2/AM also enable
    the determination of 50 β-lactamses in a cell
Construction of Reporter Gene
                                      (Boulin et al., 2006)




      Transcriptional Reporters




         Translational Reporters




    Smg-1 Based Transcriptional reporters
Ideal Bioreporter Protein and their Detection
Reporter protein        Reporter          origin           Substrate        Detection
                        genes                                               method
 Bacterial luciferase    Lux AB      Bioluminescent         O2, FMNH2       Bioluminescence
                           or            bacteria          and long chain
                        luxCDAB                              aldehyde
                            E
  β-galactosidase         lacZ            E.coli           Galactopyranos   Chemiluminesce
                                                                 ide         nc, colorimetry,
                                                                            electrochemistry
                                                                            and fluorescence
 Fluorescent protein      gfp       Aequorea victoria           NA           Fluorescence
 Infrared fluorescent    various   Bacteriophytochrome          NA           Fluorescence
       proteins                            family
     FMN based           various    Engineered from            None          Fluorescence
fluorescent proteins               Bacillus subtilis and
                                         P. putida

    β-lactamases           bla            E.coli            Lactamides        Colorimetric
   Spheriodenone          crtA        Rhodovulum           Dimethylsphero     colorimetric
                                      sulfidophilum            idene
Selection of Promoter
 • Sensitivity & specificity for the chemicals considered




Specificity
Degree to which the expression cassette is responsive towards one
specific compound not to other
Affinity of the regulatory system, driving the reporter gene through
interaction with the promoter
Stresses, induced lesions, side products by toxicological reaction
    Group specific
    Compound specific
    Metabolite specific reporter
Sensitivity of Promoter
•   Level of compound generates a significant signal which can be
    detected or measures comparable to LOD/LOQ

•   System determines the sensitivity by cellular up take & affinity of the
    compound for the regulatory system

•   E.coli possess different system for uptake of compound

     – Hydrophobic- diffusion

     – Hydrophilic - porins

•   Affinity of the compound to the regulatory protein determines the level
    of protein/ compound complex induces the cellular promoter

     – Higher affinity, lower the compound and higher sensitivity
Bacterial Bioreporter Design

Existing signaling pathway monitored by artificial output

Reporter protein is artificially controlled by sensory
regulatory system

To detect chemical compound or sample toxicity

Other possibilities for Bioreporters is oscillators or
riboregulated transcriptional cascade counter
Toxicity Bioreporter Design

 Promoter-reporter fusion


 Recombination & repair protein A (Rec A) – Lex A

  regulated SOS response

 SOS response network in E.coli & S. typhimurium induces

  toxicity response inducible gene expression–umu C, recN,
  sfiA, rec A and colicin D gene
Heat shock response to detect compound leading to protein damage –
dnaK, grpE, and lon reporter construction

Antoxoidative defense regulons – oxy R and soxRS
                                            New      toxicity      inducible
                                            promoters
                                            E.coli
                                            Shotgun chromosomal library of
                                            random 1.8kb fragment fused




                                  Reporter Protein

                  Lux CDABE
                 reporter gene
Design Of Compound Specific
                  Bioreporters
•   Isolated from bacteria displaying resistance mechanisms to specific
    compounds or metabolize that toxic compounds         Gene
                                               Regulatory gene

                    Promoter   Reporter gene




                                                                      Reporter gene

                                               Regulatory
                                                protein


       Regulatory        Reporter
        protein          protein
                                                        Reporter
                                                        protein

                                                             (Van der Meer et al., 2010)
Bioreporters for mercury & arsenic




                         (Merulla et al., 2012)
Bioreporter for Mercury


                                                 Hg2+      Mercuric      Secondary
                Activator                     transport   reductase       regulator
               repressor




                      mer R           mer T    mer P mer C    mer A       mer D

                                  O/P
             Repressor
Activation
                                                               Reporter gene
                              Mer R


               Hg2+

                                                                      Reporter        Signa
                              Mer R/Hg                                protein           l
Bioreporters for Heavy Metals
 Analyte        promoter           Reporter        Bacteria     Time for    Detection limit
                                                                detection

Aluminiu,    fliC (E. coli)   luxAB (V. harveyi)     E. coli     20 min      40–400 mM
Antimonit,   arsRD’           lacZ                   E.coli       17 h        100 mM
Arsenite
Arsenate,    arsRDABC,        luxAB (V. harveyi)   S. aureus       1h       ca. 0.01–10 mM
 arsenite    arsRBC
             E. coli, S.
             aureus)          luc (firefly)
             arsR

Cadmium      cadA (S.         luxAB (V. harveyi)   S. aureus,    1–2 h        1–100 mM
             aureus), cadA,   blaZ                  E. coli
             cadC                                  S. Aureus      1.5 h      0.5–100 mM
             (S. aureus)      luc (firefly)
             cadCo/p                               B. cereus       3h           10nM

Inorganic    mer (Tn21)       Luc (firefly)          E.coli                    <0.1FM
 mercury     Mer (Tn21)       luxAB(V. haevey)       E.coli      2-3min         10-8M
                              Lux CDABE
             Mer (Tn21)                              E.coli      40 min        0.5-5 µM
Bioreporter For Organic Chemicals
•   Direct or indirect intracellular reaction of catabolic regulatory proteins

•   Genetic dissection of pathways helped to disclose the different
    compound recognition specificities of the proteins can be exploited




                                                         P. Fluorescence 5 R (nah+, sal+)
Compound Specific Bioreporter

• Report circuit based on LysR-type transcriptional activators
  (NahR)

• Environmental compound concern are toluene, xylenes, &
  ethyl   benezene   (XylE   or   TbuT),   phenols   (DmpR),
  hydroxylated biphenyls (HbpR), Phenathathrene (PhnR)
Bacterial Reporter Construction
 Sensors protein      Host         Promoter-        Chemical        Detection
                     chassis        reporter         targets        sensitivity
                                     fusion
XylR of P. putida     E. coli       Pu-lucFF     Benzene, toluene     40 µM
                                                 & Xylene
DmpR of P. putida    P. putida      Po-luxAB     Phenol               3 µM

FruR of E.          E. herbicola    fruBp-gfp    Fructose &           2 µM
herbicola                             (AAV)      sucrose
AraC of E.coli         E.coli      pBAD-gfpuv    L-arabinose          0.5 µM
ArsR of E.coli         E.coli      arsRp-luxAb   Arsenite &            5 nM
                                                 antimonite
MerR of E.coli         E.coli        merTp-      Hg2+                  1 nM
                                   luxCDABE
CadC of S. aureus     Bacillus     cadCp-lucFF   Cd2+, Pb, Sn and      3 nM
                      subtilis                   Zn
Bioreporters for different environment
   Sensors        Host chassis   Promoter-        Chemical      Detection
   protein                        reporter         targets      sensitivity
                                   fusion

ZntR of E.coli    E.coli           zntAp-      Zn, Pb and Cd      5, 0.7µM
                                 luxCDABE                        and 10nM
                                                                respectively

TetR of E. coli   E.coli           TetAp-      Tetracycline        45nM
                                 LuxCDABE

MphR of E.coli    E.coli         mphAp-lacZ    Macrolides          10µM
SOS response      B. subtilis    yorBp-lucFF Various               60 nM
proteins of B.                               antibiotics (ex.
subtilis                                     Ciprofloxacin)

Ada of E.coli     E.coli           alkAp-      DNA alkylating      70 nM
                                 luxCDABE      agents
Bioreporter application in different
                          Environment
 •    Simple laboratory principle for the functioning
 •    Complex real world samples is more challenging
       – Presence of inhibitory compound
       – unknown compounding effect of chemical mixture
     Sensor       Host      Promoter-     Chemical       Detection      Matrix
     protein                 reporter      target          limit
                              fusion
HbpR of E.coli    E.coli   hbpR-luxAB   Hydroxylated        --       Human serum,
                                        polychlorinate                  urine
                                        d biphenyl
ArsR of E.coli    E.coli   arsR-luxAB   Arsenic           40–400     Rice powder,
                                                            mM       portable water
                                                                        (10ppb)
TetR of E.coli    E.coli   tetR-        Tetracycline      100ppb          milk
                           luxCDABE
NahR of P.          P.   nahR-luxAB     naphthalein        10nM        Soil, Gas,
putida            putida                                             aqueous phase
Next generation Bioreporters
Bioreporter cells immobilized on Silicon based CMOS surface to detect the
bioluminescence
Cells deposited on to the photodiodes, light emitting diodes or field effect
transistors
Hydrogels and other polymers used for long term maintenance of viability
Microarrays of living E.coli GFP reporter cells in PEG diacryliate Hydrogels with
optical trap




         Bioluminescent bioreporter integrated circuit sensors
Commercially Available Bioreporters
• umu-Chromo Test kit, for rapid detection of genotoxicity
  or DNA damage (ISO/ CD 13829)
• Microtox test (US EPA & ISO 11348) – natural
  bioluminescence based method
Future Prospects
• Synthetic biology approach for further streamline the
  construction and engineering of new reporter strains

• Multistrain bioreporter assay for addressing the effects of
  chemical mixtures

• Predictive performance in comparison with standards
  techniques

• Preservation of bioreporter cells in active form

• Regulatory issues limiting the bioreporter assay
Conclusions
 Based on gene expression in presence of toxic/ stress, heavy metals
   antibiotics, organic compounds etc exploited for construction of
   Bioreporters by fusion of specific reporter gene with promoter
 Assaying more complex real sample is more challenging, because of
   possible presence of inhibitory compounds, unknown compounding
   effects on behaviors & sportive effect
 Bioreporters also explored in foodstuffs for the detection of arsenic in rice
   and tetracycline residues in milk below 100ppb
 Technical hurdle for limiting the application bioreporter assay is limiting
   use of genetic modification of the reporter cell
 Overcome this barrier it is imperative that the bioreporter tests are
   accredited as internationally accepted test
Raghu H V & kumar N.

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Raghu H V & kumar N.

  • 1. Design of Bacterial Bioreporters for Their Application in Assays of Harmful Chemicals in Different Environment Raghu H V & Kumar N.
  • 2. Introduction Physico-chemical analysis  High selectivity, sensitivity, accuracy and reproducibility  Drawbacks–  Limited to predetermined set of substances,  Fails to indicate bioavailability  Time consuming, expensive & requires lot of expertise
  • 3. Bioreporters • Measures Bioavailable concentration • Predict the fate & availability • Cost effective • Multianalyte approach • Detects group of compound rather single analyte
  • 4. What are Bioreporter? A microorganisms, cell culture or cell line, often genetically engineered, with an activity that reflects changes in environmental conditions in dose response dependent manner Signal Transcription Translation Promoter Reporter m RNA Reporter gene protein Analyte
  • 5. Principle of Bacterial Bioreporters Analyte Bacterial Signal Bioreporters Molecular recognition or Physico-chemical condition Class I Class II Class III Target Stress Compound compound- Increase in the or Stress Increase in the out put decrease in out put the out put (van der Meer et al., 2004)
  • 6. Cont… Analyte RNA degraded to polymerase effector Periplasmic Regulator Analyte A binding A protein binds analyte A operator promoter Reporter Transport/ Regulator recruits/ activates Analyte Diffusion Diffusion RAN polymerase binds to regulator A operator promoter Reporter Signal Reporter protein synthesized A mRNA Reporter protein, quantum operator promoter Reporter yield, CM stability, specific Cytosol activity out (van der Meer et al., 2004)
  • 7. Fundamentals of Bioreporter Promoter Transcription Translation Lights On Reporter m RNA gene Reporter protein Analyte or stress Transcription Lights Transcription off Toxic Translation Promoter Reporter gene Reporter Transcription protein No Translation Toxic Analyte Lights On (Xu et al., 2012)
  • 8. Reporter gene Firefly luciferase (luc) Bacterial luciferase (lux) Green fluorescent protein (GFP) Chloramphenicol acetyltransferase (CAT) Aequorin Uroporphyrinogen III methyltransferases β-galactosidase β-lactamase Alkaline phosphatase (SPAP) (New et al., 2003)
  • 9. Firefly Luciferase (luc)  luc gene derived from Photinus pyralis  High light out and rapid response kinetics Mg2+ luciferase + luciferin + ATP Luciferase. luciferyl-AMP + PPi Luciferase. luciferyl-AMP + O2 luciferase + oxyluciferin + AMP + C02 + hv Exogenous addition of luciferin substrate Not able to react autonomously or monitor Maximal light output translates into very sensitive assay
  • 10. Luciferase (lux gene) (Close et al., 2009)
  • 11. lux Gene • lux AB genes – Encodes only luciferase – Exogenous addition of aldehyde (n-dacanol) – Brighter & easier signal • lux CDABE genes – Continuous substrate independent signaling – Accommodate complete gene cassettes – Contains full complement of luciferase-luciferrin complex – Real time to near real time capabilities • lux CDABE operon synthetically optimized away from its native AT rich state to towards GC rich MO’s
  • 12. Green Fluorescent Protein (GFP) Photoprotein clone from jelly fish Aequorea Victoria Doesn't require any substrate and dependent on external light source Functioning semi-continuously and near real time Dual color formats at different spectra
  • 13. Fluorescent Reporter Protein in Array System Protein Excitation Emission GFP 395 509 EGFP 488 509 BFP 380 440 GFPuv 395 509 YFP 513 527 CFP 433 475 CobA 357 605 RFP 558 583
  • 14. Aequorin Ca2+ sensitive luminescent protein – Aequorea aequorea - Inhibited by Mg2+ and also triggered by Eu2+, Sr2+ and Ba2+ Multifaceted reporter protein with Affinities (KD) 1-10µL
  • 15. Chloramphenicol Acetyltransferase (CAT) CAT gene Acetyl coenzyme A + Chloramphenicol CoA + CAP-3 Acetate • Radiolabelled (14 C or 3H) CAP by autoradiography & liquid scintillation counting • Fluorescent measurement • Ex: CAT TOX (L) assay
  • 16. β-Galactosidase • LacZ gene from E.coli encodes a β-Galactosidase enzyme • Hydrolysis of β-galactoside disaccharide into monosaccharide yield colorimetric signal • SOS chromotest – LacZ fusions to DNA to monitor mutagenic/ Carcinogenic genotoxic compound • Luminescent, chemiluminescent or fluorescent endpoint also possible • Contribute to elevated background signal • Delayed data accumulation
  • 17. Uroporphyrinogen (Urogen) III Methyltransferases (UMT)  Important for the biosynthetic pathways of vitamin B12 and siroheme  Vitamin B12 - cobA genes in Bacillus megatarium, Methanobacterium ivanovii, Propionibacterium freudenreichii, and Pseudomonas denitrificans.  Second form of UMT is encoded by the cysG gene in E. coli and S. typhimurium.  Bioreporter for the selection of recombinant plasmids, as a marker for gene transcription, and for the detection of toxic salts such as arsenite and antimonite. 300 nm Red to red- orange
  • 18. β-lactamases • Cleaves penicillin and cephalosporin • TEM-1 β-lactamses (E.coli) engineered into cytosolic membrane associated forms • Membrane permeable flourogenic substrate CCF2/AM also enable the determination of 50 β-lactamses in a cell
  • 19. Construction of Reporter Gene (Boulin et al., 2006) Transcriptional Reporters Translational Reporters Smg-1 Based Transcriptional reporters
  • 20. Ideal Bioreporter Protein and their Detection Reporter protein Reporter origin Substrate Detection genes method Bacterial luciferase Lux AB Bioluminescent O2, FMNH2 Bioluminescence or bacteria and long chain luxCDAB aldehyde E β-galactosidase lacZ E.coli Galactopyranos Chemiluminesce ide nc, colorimetry, electrochemistry and fluorescence Fluorescent protein gfp Aequorea victoria NA Fluorescence Infrared fluorescent various Bacteriophytochrome NA Fluorescence proteins family FMN based various Engineered from None Fluorescence fluorescent proteins Bacillus subtilis and P. putida β-lactamases bla E.coli Lactamides Colorimetric Spheriodenone crtA Rhodovulum Dimethylsphero colorimetric sulfidophilum idene
  • 21. Selection of Promoter • Sensitivity & specificity for the chemicals considered Specificity Degree to which the expression cassette is responsive towards one specific compound not to other Affinity of the regulatory system, driving the reporter gene through interaction with the promoter Stresses, induced lesions, side products by toxicological reaction Group specific Compound specific Metabolite specific reporter
  • 22. Sensitivity of Promoter • Level of compound generates a significant signal which can be detected or measures comparable to LOD/LOQ • System determines the sensitivity by cellular up take & affinity of the compound for the regulatory system • E.coli possess different system for uptake of compound – Hydrophobic- diffusion – Hydrophilic - porins • Affinity of the compound to the regulatory protein determines the level of protein/ compound complex induces the cellular promoter – Higher affinity, lower the compound and higher sensitivity
  • 23. Bacterial Bioreporter Design Existing signaling pathway monitored by artificial output Reporter protein is artificially controlled by sensory regulatory system To detect chemical compound or sample toxicity Other possibilities for Bioreporters is oscillators or riboregulated transcriptional cascade counter
  • 24. Toxicity Bioreporter Design  Promoter-reporter fusion  Recombination & repair protein A (Rec A) – Lex A regulated SOS response  SOS response network in E.coli & S. typhimurium induces toxicity response inducible gene expression–umu C, recN, sfiA, rec A and colicin D gene
  • 25. Heat shock response to detect compound leading to protein damage – dnaK, grpE, and lon reporter construction Antoxoidative defense regulons – oxy R and soxRS New toxicity inducible promoters E.coli Shotgun chromosomal library of random 1.8kb fragment fused Reporter Protein Lux CDABE reporter gene
  • 26. Design Of Compound Specific Bioreporters • Isolated from bacteria displaying resistance mechanisms to specific compounds or metabolize that toxic compounds Gene Regulatory gene Promoter Reporter gene Reporter gene Regulatory protein Regulatory Reporter protein protein Reporter protein (Van der Meer et al., 2010)
  • 27. Bioreporters for mercury & arsenic (Merulla et al., 2012)
  • 28. Bioreporter for Mercury Hg2+ Mercuric Secondary Activator transport reductase regulator repressor mer R mer T mer P mer C mer A mer D O/P Repressor Activation Reporter gene Mer R Hg2+ Reporter Signa Mer R/Hg protein l
  • 29. Bioreporters for Heavy Metals Analyte promoter Reporter Bacteria Time for Detection limit detection Aluminiu, fliC (E. coli) luxAB (V. harveyi) E. coli 20 min 40–400 mM Antimonit, arsRD’ lacZ E.coli 17 h 100 mM Arsenite Arsenate, arsRDABC, luxAB (V. harveyi) S. aureus 1h ca. 0.01–10 mM arsenite arsRBC E. coli, S. aureus) luc (firefly) arsR Cadmium cadA (S. luxAB (V. harveyi) S. aureus, 1–2 h 1–100 mM aureus), cadA, blaZ E. coli cadC S. Aureus 1.5 h 0.5–100 mM (S. aureus) luc (firefly) cadCo/p B. cereus 3h 10nM Inorganic mer (Tn21) Luc (firefly) E.coli <0.1FM mercury Mer (Tn21) luxAB(V. haevey) E.coli 2-3min 10-8M Lux CDABE Mer (Tn21) E.coli 40 min 0.5-5 µM
  • 30. Bioreporter For Organic Chemicals • Direct or indirect intracellular reaction of catabolic regulatory proteins • Genetic dissection of pathways helped to disclose the different compound recognition specificities of the proteins can be exploited P. Fluorescence 5 R (nah+, sal+)
  • 31. Compound Specific Bioreporter • Report circuit based on LysR-type transcriptional activators (NahR) • Environmental compound concern are toluene, xylenes, & ethyl benezene (XylE or TbuT), phenols (DmpR), hydroxylated biphenyls (HbpR), Phenathathrene (PhnR)
  • 32. Bacterial Reporter Construction Sensors protein Host Promoter- Chemical Detection chassis reporter targets sensitivity fusion XylR of P. putida E. coli Pu-lucFF Benzene, toluene 40 µM & Xylene DmpR of P. putida P. putida Po-luxAB Phenol 3 µM FruR of E. E. herbicola fruBp-gfp Fructose & 2 µM herbicola (AAV) sucrose AraC of E.coli E.coli pBAD-gfpuv L-arabinose 0.5 µM ArsR of E.coli E.coli arsRp-luxAb Arsenite & 5 nM antimonite MerR of E.coli E.coli merTp- Hg2+ 1 nM luxCDABE CadC of S. aureus Bacillus cadCp-lucFF Cd2+, Pb, Sn and 3 nM subtilis Zn
  • 33. Bioreporters for different environment Sensors Host chassis Promoter- Chemical Detection protein reporter targets sensitivity fusion ZntR of E.coli E.coli zntAp- Zn, Pb and Cd 5, 0.7µM luxCDABE and 10nM respectively TetR of E. coli E.coli TetAp- Tetracycline 45nM LuxCDABE MphR of E.coli E.coli mphAp-lacZ Macrolides 10µM SOS response B. subtilis yorBp-lucFF Various 60 nM proteins of B. antibiotics (ex. subtilis Ciprofloxacin) Ada of E.coli E.coli alkAp- DNA alkylating 70 nM luxCDABE agents
  • 34. Bioreporter application in different Environment • Simple laboratory principle for the functioning • Complex real world samples is more challenging – Presence of inhibitory compound – unknown compounding effect of chemical mixture Sensor Host Promoter- Chemical Detection Matrix protein reporter target limit fusion HbpR of E.coli E.coli hbpR-luxAB Hydroxylated -- Human serum, polychlorinate urine d biphenyl ArsR of E.coli E.coli arsR-luxAB Arsenic 40–400 Rice powder, mM portable water (10ppb) TetR of E.coli E.coli tetR- Tetracycline 100ppb milk luxCDABE NahR of P. P. nahR-luxAB naphthalein 10nM Soil, Gas, putida putida aqueous phase
  • 35. Next generation Bioreporters Bioreporter cells immobilized on Silicon based CMOS surface to detect the bioluminescence Cells deposited on to the photodiodes, light emitting diodes or field effect transistors Hydrogels and other polymers used for long term maintenance of viability Microarrays of living E.coli GFP reporter cells in PEG diacryliate Hydrogels with optical trap Bioluminescent bioreporter integrated circuit sensors
  • 36. Commercially Available Bioreporters • umu-Chromo Test kit, for rapid detection of genotoxicity or DNA damage (ISO/ CD 13829) • Microtox test (US EPA & ISO 11348) – natural bioluminescence based method
  • 37. Future Prospects • Synthetic biology approach for further streamline the construction and engineering of new reporter strains • Multistrain bioreporter assay for addressing the effects of chemical mixtures • Predictive performance in comparison with standards techniques • Preservation of bioreporter cells in active form • Regulatory issues limiting the bioreporter assay
  • 38. Conclusions  Based on gene expression in presence of toxic/ stress, heavy metals antibiotics, organic compounds etc exploited for construction of Bioreporters by fusion of specific reporter gene with promoter  Assaying more complex real sample is more challenging, because of possible presence of inhibitory compounds, unknown compounding effects on behaviors & sportive effect  Bioreporters also explored in foodstuffs for the detection of arsenic in rice and tetracycline residues in milk below 100ppb  Technical hurdle for limiting the application bioreporter assay is limiting use of genetic modification of the reporter cell  Overcome this barrier it is imperative that the bioreporter tests are accredited as internationally accepted test