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PLANT/SOIL CAPACITIES TO REMOVE HARMFUL SUBSTANCES FROM
POLLUTED INDOOR AIR
R.A.Wood, M.D.Burchett RA Orwell, J Tarran, F Torpy
Plants and Environmental Quality Group, Centre for Ecotoxicology, UTS,
Westbourne St, Gore Hill, NSW 2065
Australia


The aesthetic value of indoor plants is easily seen, however the unseen ability of
indoor plants to improve indoor air quality has never been conclusively shown or,
until now, quantified.
Research at the University of Technology, Sydney has shown that indoor plants do
improve air quality. As a result, clear claims can now be made as to how indoor plants
improve air quality, and development of varieties with an even better capacity for
improving indoor air can begin.


Why worry about indoor air quality?


Could everyday activities in our homes and offices, places we usually consider to be
essentially unpolluted, expose us to the greatest contact with potentially toxic air
pollutants?


Could ordinary consumer products such as air fresheners, deodorisers, household
pesticides, cleaning compounds and various building furnishings and materials be
more of a threat to our health than industrial pollution? The short answer to these
questions is yes!


The ongoing development of new materials and products has substantially enhanced
our standard of living. In our homes and offices, modern building materials,
insulation, glues, fabrics, carpets, cleaning materials, personal care products and
pesticides, often expose us to a wide spectrum of chemicals in the air we breathe. The
presence of these chemicals, even at very low levels is now known to influence indoor
air quality with potentially adverse affects on our health. More than 300 different
volatile organic compounds have been identified in office air. Exposure to these
pollutants is suspected as the major cause of the headaches, lethargy, sore eyes and
respiratory problems experienced by some office workers. There is an increasing
awareness of the costs to our health, the environment and even to productivity.


We tend to take for granted the air we breathe both outdoors and indoors, particularly
indoor air if it is “conditioned.” Our perception of air quality is influenced by our
sense of smell and to a lesser extent visually. This perception can be misleading; our
senses may not be able to detect pollutants in trace amounts that are harmful to our
health. When exposed to an odour for a period of time the perception of the odour is
diminished as our olfactory cells tire very easily. Our lungs are our most important
point of contact with the outside world. We may drink 2 litres of liquid each day but
we breathe in approximately 6 to 10 litres of air every minute, around 15,000 litres
per day. Most urban dwellers usually spend about 80% or more of the time indoors, so
the quality of indoor air becomes a major health consideration.


Plants as decontaminators


Outdoor plants are known to absorb air and soil pollutants and detoxify them. Plants
and soil microorganisms are used, for example, in the remediation of contaminated
soils. Previous screening studies have shown that some ‘indoor’ plants can also
reduce concentrations of air-borne VOCs and suggested that the microorganisms of
the soil might also be involved.


We compared the VOC removal performance of three top-selling indoor plant
species, Howea forsteriana (Kentia palm), Spathiphyllum wallisii var. Petite (Peace
Lily), and Dracaena deremensis var. Janet Craig. Benzene (a carcinogen) and n-
hexane (a neurotoxin) were chosen as the test VOCs, because they are common in
indoor air.


Findings


Overall all three species were found to be effective removers of both VOCs There
were strong similarities in response among the plant species and with both VOCs,
although differences between species were also found (Figs 1-2).
60       Kt.Bz.Pmx
                  50                                                                  5
                                                    L/D
                  40                                                                                         PR        6
                  30
                           1 2                     3 ↓4                                                      ↓
                  20
                  10
                   0
        Benzene
         ppm 60        0                       5               10                   15    Day          20                  25
                50                       L/D            Kt.Bz.Hyd                                            Note : Two
                                                   PR                                              5
                40                       ↓                                                                   complementary
                           1 2
                30                      3 4        ↓6                           12        3                  experiments shown
                20                                                                                           for Kt.Bz.hyd
                10
                 0
                       0                       5               10       0                     5                  10
                                                                                Day

                  50                Sp.Bz.Pmx                                         5
                  40                                                  L/D
                  30           1                                    3 ↓4
                  20                       2
                  10
                   0
        Benzene
         ppm                       Sp.Bz.Hyd
                  50                                                        5
                                                          L/D
                  40                                                                                   PR
                  30           1                        3↓ 4
                                                                                                        ↓ 6
                  20                2
                  10
                   0

                       0                           5                10                        15                  20             25
                                                                                Day

                50                                                              5
                           Dc.Bz.Pmx
                40                                                                   PR       6
                           1                               3
                30                                                                   ↓
                                   2
                20
                10
         Benzene 0
          ppm
                  50           Dc.Bz.Hyd                            5
                  40                            L/D                                                         PR
                  30       1           2       3 ↓                                                          ↓ 6
                                                    4
                  20
                  10
                   0

                       0                       5               10
                                                                            Day 15                          20             25


Fig.1. Benzene (Bz) levels in test chambers during experiments with three indoor plant species.
        Step increments in VOC concentration correspond to injections of benzene Kt = Kentia
        (Howea forsteriana); Sp = Spathiphyllum var, Petite; Dc = Dracaenae deremensis; Pmx =
        potting mix; Hyd = hydroponics; L/D =change from light to dark; PR = plant removed and
        used substrate or medium returned to chamber. Each point mean ± SEM (n = 4).
180                   Kt.Hx.Pmx
                    160                                                                 5
                    140                                                      L/D                      6
                                    1                               3           4
                    120                                                      ↓                PR
                    100                                                                       ↓
                     80
                     60                               2
                     40
              Hexane 20
               ppm    0
                                         Kt.Hx.Hyd                           L/D            PR
                     120            1                               3        ↓ 4                          6
                     100                          2                                         ↓
                      80
                      60
                      40
                      20
                                0                             5                    10                         15                 20
                                                                                        Day
                     100        1
                                        Sp.Hx.Pmx
                      80
                      60                              3
                                         2
                      40
                     220
                       20
                        0
              Hexane                                                                                  5
               ppm 140                  Sp.Hx.Hyd                                                                     PR
                     120                                                       L/D
                                1                                            3 ↓ 4                                    ↓
                     100                          2                                                                          6
                      80
                      60
                      40
                            0             5               10            15        20             25            30      35         40
                                                                             Day

                   160              Dc.Hx.Pmx                                                             5
                   140                                                                 L/D                            PR
                   120          1                                             3           4                              6
                   100                                                                 ↓                              ↓
                    80                            2
                    60
                    40
             Hexane 20
                      0
              ppm                   Dc.Hx.Hyd
                    120         1                                                                             L/D
                    100                                                                                           4
                                                                                  3                           ↓
                     80                                   2
                     60
                     40
                     20
                      0
                            0                 5                10            15             20                25      30          35
                                                                                  Day



Fig.2. n-hexane (Hx) levels in test chambers during experiments with three indoor plant species.
Step increments in VOC concentration correspond to injections of n-hexane. Kt = Kentia (Howea
forsteriana); Sp = Spathiphyllum var., Petite; Dc = Dracaena deremensis; Pmx = potting mix.
We then tested three other widely used species, Epipremnum aureum (Devil’s Ivy),
Schefflera ‘Amate’ (Queensland umbrella tree) and Spathiphyllum ‘ Sensation’ with
similar results.
Like most research projects, the findings unfolded like a detective story – following
clues and piecing together the evidence.




What happens with the first dose of VOC?


Since we had to start somewhere, each experiment was commenced in continuous
light, such as can be found in offices, hotels or shopping malls. Immediately after
applying the first dose of VOC the removal rates were very slow. However, within a
fairly short time (1-2 days for benzene; 4-5 days for n-hexane) they accelerated
markedly. This increase in rate was in response to a ‘taste’ of the VOC. It involves
the ‘switching on’ (ie induction) of a biochemical system to deal with the compound
(consume / metabolise it). With further topping-up doses with either VOC this
induced removal activity was maintained, or even increased further. That is, they get
better with practice!


Is light necessary for VOC removal?


To test this question, plants were then transferred to continuous dark (lights off, black
plastic over chambers).      It is well known that under these conditions plant
photosynthesis stops, so metabolic activity will be largely reduced to baseline ‘dark’
respiration.   Stomates will also be shut, so there will be virtually no gaseous
absorption into the leaves. What happens now? Does VOC removal slow down? No!
The process kept on going at the same sorts of rates as in the light (Figs 1-2). In
addition, when (still in the dark), new doses of VOC were injected, at even higher
concentrations, (ie raised from 25 to 50 ppm for benzene and from 100 to150 ppm for
n-hexane), the removal rates usually increased further as well. This indicates that
with each plant species, the system remained fully operative under dark conditions,
and in fact could respond to, and cope with, higher doses of each compound. In other
words, we had not yet arrived at concentrations high enough to saturate the
biochemical removal system (and that aspect still remains to be investigated further).
What are the relative roles of the plant and soil micro-organisms, in the removal
process?


Was it the plant itself that was directly responsible for the VOC removal, even in the
dark? To answer this, we removed the plants, replaced the potting mix into the pots,
and put the pots back into the chambers. New standard doses of the VOC were then
applied. Again, the VOC continued to disappear at rates comparable with, though
generally slightly less than, those found prior to the plant's removal (Figs 1-2). After
the plant’s removal, experiments were sometimes continued for a further 7 - 10 days,
with top-up doses as required, and the activity was maintained in every case.


The sustained activity with further doses, and in the absence of the plant, tells us two
things: First, the continued activity confirms that this is a true biological response, and
not merely an adsorption / absorption process. Secondly, it shows that it must be the
micro-organisms of the potting mix that are the ‘rapid-removal agents’ of the pot-
plant system. The plant is somehow involved, however, as discussed below.


What happens when the plant is transferred to hydroponics?


This was to test the plant removed from the potting mix. The roots were thoroughly
washed in sterile water to remove particles of the potting mix and if possible some of
the micro-organisms clinging to the surface of the roots. Nevertheless, some VOC
removal sometimes continued to occur in hydroponic medium (Figs.1-2). Sometimes,
though not always, the system achieved the same removal rates as in the potting mix.
This suggests that the microorganisms are at least in some cases fairly firmly attached
onto or inside the roots. The differences in response among the plant species in this
medium suggest different relationships between the plant and the microorganisms
associated with the root systems.
What happens when unplanted potting mix is dosed with VOC?


Tests with watered new potting mix, that had not been used to grow plants, showed a
very slow induction when dosed with VOC, and the final induced activity was
estimated to be only about half of that with plants (Fig. 3). In addition, there was
some evidence of the system becoming exhausted. The results confirm what is
known of potting mixes generally, namely that they contain a supply of
microorganisms before plants are introduced. However, the results also suggest that
the readily available nutrients for microbial growth and reproduction in the potting
mix will not last very long in the absence of a growing plant.




                             Pmx Control Expt.
                             (plants absent throughout).
                  30
                             1                      3
                  25
          Benzene
           ppm    20                 2
                  15
                  10
                   5
                   0
                         0                    5            10
                                                     Day

Fig.3. Benzene (Bz) levels in test chamber during control experiment with
"virgin" potting mix, ie. potting mix which not previously used as substrate for
plants. Each point mean ± SEM (n = 4).




The bottom line – a new and improved marketing message



Indoor pot plants can now be confidently promoted as helping to improve the quality
of the indoor environment. The way of the future will certainly be to use them
routinely for that purpose, and to ensure that buildings are designed to exploit their
usefulness for clean air as well as for their living beauty! In summary, we can safely
state that:


1.      The pot-plant system really does remove VOCs from indoor air!


2.     The system gets better on exposure to VOCs and maintains performance with
       repeated doses.


3.     From 3 to 10 times the maximum permitted Australian occupational indoor air
       concentrations of each compound can be removed within about 24 hours, under
       light or dark conditions without saturating the system.
4.     The pot plant system can also remove very low residual concentrations as well,
-
-      The fact that similar responses were found with the three plant species, under
       all of the test conditions, indicates two things: (a), that this is a general plant-
       soil phenomenon, that is, it can be expected to be found with any pot-plant
       species; and (b) that it is the micro-organisms of the growth medium which
       play a primary role as the 'rapid-response agents' in VOC removal in the
       potted-plant system.
-      The plants are also involved. Comparisons of performance among the three
       plant species indicate that they have different substrate microbiological
       populations, and / or that there are different relationships between the
       microorganisms and the roots of the particular species. The results with new
       potting mix also indicate the nourishing role of the plant in promoting
       microbial growth.
It is well established from research with crop species that different plant species
develop a species-specific soil flora around their roots, producing a symbiotic
microcosm of activity. It is also known that plants expend energy nourishing their
substrate microorganisms, sometimes secreting from 25 to 45% of their net
photosynthetic product from their roots to keep the microbes growing.
Further work


We are now working on two follow-up projects. The first is an investigation into
which microorganisms, associated with these plant species and growth media, are
involved in the VOC removal process. This will enable the horticultural development
of plant-and-soil varieties and systems with enhanced clean-air capabilities. The
second project is on the testing of these and other interior foliage plant species under
flow-through conditions, to seek answers crucial questions about how much plant
material, of which species will make the most impact on improving indoor air quality
in the ‘real world’. For this project we will be using both test chambers of the same
size as those used in the static experiments, and a scaled-up, room-sized dynamic
chamber, in collaboration with associate investigator Dr. Steven Brown, at the Air
Quality Laboratory of CSIRO, Melbourne.




Acknowledgments


We thank the Flower Council of Holland, the Horticultural Research and
Development Corporation of Australia and the Nursery Industry Association of NSW
via the Horticultural Stock and Nurseries Act (NSW Agriculture), for funds for this
project. Thanks also to the Interior Plantscapers Association of NSW, HousePlants
Australia and the Lord Howe Island Board, for plant materials and continuing interest
and assistance. We also thank Ms Narelle Richardson, Laboratory Manager, and other
staff and students of the Department of Environmental Sciences, UTS who have
assisted in this project.


References and further reading
-    When You Can’t Breathe, Nothing Else Matters. American Lung Association
     (1996), NY.
-      Bascom R., 1997. Plenary Paper: Health and Indoor Air Quality in Schools.
       Proceedings of Healthy Buildings / IAQ '97, Washington DC, 27 Sept. - 2 Oct.
       1997, Vol. 1, 3-12.
-   Indoor Air Quality, Australia: State of the Environment Technical paper series
    (Atmosphere), Brown, SK, 1997, (a). Dept. Environment, Sport and Territories,
    Canberra.
-   Volatile organic compounds in indoor air: sources and control. Brown, SK,
    1997, (b). Chemistry in Australia, Jan / Feb, 10-13.
-   Concentrations of volatile organic compounds in indoor air – a review. Brown,
    SK, Sim, MR, Abramson, MJ and Gray, CN, 1994.                 Indoor Air 4: 123-
    134.1994;
-   Home and workplace: complaints and symptoms in office workers and
    correlation with indoor air pollution. Carrer, P, Alcini, D, Cavallo, D, Visigalli,
    F, Bollini, D and Maroni, M, 1999.          In, Proceedings of 8th international
    Conference on Indoor air Quality and Climate, Edinburgh, Scotland, 129-134.
-   Pilot Study to Assess the Impact of Green Plants on NO2 levels in Homes.
    Coward M, Ross D, Coward S, Cayless S and Raw G, 1996. Building Research
    Establishment Note N154/96. Watford, UK.
-   Detoxification of formaldehyde by the Spider Plant (Chlorophytum comosum
    L.) and by soybean (Glycine max L.) cell suspension cultures. Giese, M., Bauer-
    Dorancth, U, Langerbartels, C, Sandermann Jr, H, 1994. Plant Physiology 104:
    1301 - 1309)
-   Particulate matter accumulation on horizontal surfaces in interiors: influence of
    foliage plants. Lohr VI and Pearson-Mims CH, 1996.                   Atmospheric
    Environment 30: 14, 2565-2568.
-   Exposure Standards for Atmospheric Contaminants in the Occupational
    Environment. National Occupational Health and Safety Commission (Aust),
    1991. AGPS, Canberra, Australia.
-   Draft National Protection Measure and Impact Statement for Ambient Air
    Quality, NEPC (National Environment Protection Council) (1997). NEPC
    Service Corp. Adelaide p.101
-   Metropolitan Air Quality Study-Outcomes and Implications for Managing Air
    Quality. NSW EPA (1996) EPA 96/20; Chatswood NSW.
-   Proceedings of Health and Urban Air Quality in NSW Conference, Sydney June
    3-4 Vol I, II. NSW Health Dept (1996) NSW Health Dept. Gladesville NSW.
-    Air Pollution and Plant Metabolism. Schulte-Hostede S, Darrall NM, Blank
     LW and Wellburn AR (Eds), 1987 Elsevier, NY.
-   Rhizospheric hydrocarbon-utlizing microorganisms as potential contributor to
    phytoremediation for the oily Kuwait desert. Radwan, SS, Al-Awadhi, H.,
    Sorkhoh, NA and El-Nemr, IM, 1998. Microb Res 153: 3, 247 – 251.
-   Higher plant metabolism of xenobiotics; the ‘green liver’ concept. Sandermann
    H., Jr, 1994. Pharmacogenetics 4: 225-241.
-    Adsorption of naphthalene onto plant roots. Schwab, AP, Al-Assi, AA and
     Banks, MK,1998. J Environ Qual 27: 1, 220 - 224).
-   Interior Landscape Plants for Indoor Air Pollution Abatement, Final Report,
    Sept., Wolverton BC, Johnson A and Bounds K, 1989. NASA Stennis Space
    Centre MS.
-   Removal of Formaldehyde from Sealed Experimental Chambers, by Azalea,
    Poisettia and Dieffenbachia. Wolverton Environmental Services INc., 1991.
    Res. Report No. WES/100/01-91/005.
-   Eco-Friendly House Plants. Wolverton BC 1996. Weidenfeld and Nicolson,
    London.
-   Living plants to improve indoor air quality. Wood RA, Orwell RL and Burchett
    MD,1998. In, MD Burchett, J. Tarran and R Wood (eds). Towards a New
    Millennium of People-Plant Relationships, Contributions from the International
    People Plant Symposium, Sydney, Australia July. 115-122
-   Absorption of organic compounds in indoor air by commonly used indoor
    plants. Wood, R. A., Orwell, R., and Burchett, M. D., Tarran, J. and Brown,
    SK, 2000.    Proceedings of Healthy Buildings 2000, Espoo, Finland, Aug 6-
    10, Vol 2, 125-130.
-   Potted plant-growth media: interactions and capacities in removal of volatiles
    from indoor air. Wood, R. A., Orwell, R., Tarran, J., Torpy F., and Burchett,
    M. D., 2002. Journal of Environmental Horticulture and Biotechnology. 77: (1)
    120-129.

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Plant-Soil Capacities to Remove Harmful Substances from Polluted Indoor Air

  • 1. PLANT/SOIL CAPACITIES TO REMOVE HARMFUL SUBSTANCES FROM POLLUTED INDOOR AIR R.A.Wood, M.D.Burchett RA Orwell, J Tarran, F Torpy Plants and Environmental Quality Group, Centre for Ecotoxicology, UTS, Westbourne St, Gore Hill, NSW 2065 Australia The aesthetic value of indoor plants is easily seen, however the unseen ability of indoor plants to improve indoor air quality has never been conclusively shown or, until now, quantified. Research at the University of Technology, Sydney has shown that indoor plants do improve air quality. As a result, clear claims can now be made as to how indoor plants improve air quality, and development of varieties with an even better capacity for improving indoor air can begin. Why worry about indoor air quality? Could everyday activities in our homes and offices, places we usually consider to be essentially unpolluted, expose us to the greatest contact with potentially toxic air pollutants? Could ordinary consumer products such as air fresheners, deodorisers, household pesticides, cleaning compounds and various building furnishings and materials be more of a threat to our health than industrial pollution? The short answer to these questions is yes! The ongoing development of new materials and products has substantially enhanced our standard of living. In our homes and offices, modern building materials, insulation, glues, fabrics, carpets, cleaning materials, personal care products and pesticides, often expose us to a wide spectrum of chemicals in the air we breathe. The presence of these chemicals, even at very low levels is now known to influence indoor air quality with potentially adverse affects on our health. More than 300 different volatile organic compounds have been identified in office air. Exposure to these pollutants is suspected as the major cause of the headaches, lethargy, sore eyes and
  • 2. respiratory problems experienced by some office workers. There is an increasing awareness of the costs to our health, the environment and even to productivity. We tend to take for granted the air we breathe both outdoors and indoors, particularly indoor air if it is “conditioned.” Our perception of air quality is influenced by our sense of smell and to a lesser extent visually. This perception can be misleading; our senses may not be able to detect pollutants in trace amounts that are harmful to our health. When exposed to an odour for a period of time the perception of the odour is diminished as our olfactory cells tire very easily. Our lungs are our most important point of contact with the outside world. We may drink 2 litres of liquid each day but we breathe in approximately 6 to 10 litres of air every minute, around 15,000 litres per day. Most urban dwellers usually spend about 80% or more of the time indoors, so the quality of indoor air becomes a major health consideration. Plants as decontaminators Outdoor plants are known to absorb air and soil pollutants and detoxify them. Plants and soil microorganisms are used, for example, in the remediation of contaminated soils. Previous screening studies have shown that some ‘indoor’ plants can also reduce concentrations of air-borne VOCs and suggested that the microorganisms of the soil might also be involved. We compared the VOC removal performance of three top-selling indoor plant species, Howea forsteriana (Kentia palm), Spathiphyllum wallisii var. Petite (Peace Lily), and Dracaena deremensis var. Janet Craig. Benzene (a carcinogen) and n- hexane (a neurotoxin) were chosen as the test VOCs, because they are common in indoor air. Findings Overall all three species were found to be effective removers of both VOCs There were strong similarities in response among the plant species and with both VOCs, although differences between species were also found (Figs 1-2).
  • 3. 60 Kt.Bz.Pmx 50 5 L/D 40 PR 6 30 1 2 3 ↓4 ↓ 20 10 0 Benzene ppm 60 0 5 10 15 Day 20 25 50 L/D Kt.Bz.Hyd Note : Two PR 5 40 ↓ complementary 1 2 30 3 4 ↓6 12 3 experiments shown 20 for Kt.Bz.hyd 10 0 0 5 10 0 5 10 Day 50 Sp.Bz.Pmx 5 40 L/D 30 1 3 ↓4 20 2 10 0 Benzene ppm Sp.Bz.Hyd 50 5 L/D 40 PR 30 1 3↓ 4 ↓ 6 20 2 10 0 0 5 10 15 20 25 Day 50 5 Dc.Bz.Pmx 40 PR 6 1 3 30 ↓ 2 20 10 Benzene 0 ppm 50 Dc.Bz.Hyd 5 40 L/D PR 30 1 2 3 ↓ ↓ 6 4 20 10 0 0 5 10 Day 15 20 25 Fig.1. Benzene (Bz) levels in test chambers during experiments with three indoor plant species. Step increments in VOC concentration correspond to injections of benzene Kt = Kentia (Howea forsteriana); Sp = Spathiphyllum var, Petite; Dc = Dracaenae deremensis; Pmx = potting mix; Hyd = hydroponics; L/D =change from light to dark; PR = plant removed and used substrate or medium returned to chamber. Each point mean ± SEM (n = 4).
  • 4. 180 Kt.Hx.Pmx 160 5 140 L/D 6 1 3 4 120 ↓ PR 100 ↓ 80 60 2 40 Hexane 20 ppm 0 Kt.Hx.Hyd L/D PR 120 1 3 ↓ 4 6 100 2 ↓ 80 60 40 20 0 5 10 15 20 Day 100 1 Sp.Hx.Pmx 80 60 3 2 40 220 20 0 Hexane 5 ppm 140 Sp.Hx.Hyd PR 120 L/D 1 3 ↓ 4 ↓ 100 2 6 80 60 40 0 5 10 15 20 25 30 35 40 Day 160 Dc.Hx.Pmx 5 140 L/D PR 120 1 3 4 6 100 ↓ ↓ 80 2 60 40 Hexane 20 0 ppm Dc.Hx.Hyd 120 1 L/D 100 4 3 ↓ 80 2 60 40 20 0 0 5 10 15 20 25 30 35 Day Fig.2. n-hexane (Hx) levels in test chambers during experiments with three indoor plant species. Step increments in VOC concentration correspond to injections of n-hexane. Kt = Kentia (Howea forsteriana); Sp = Spathiphyllum var., Petite; Dc = Dracaena deremensis; Pmx = potting mix.
  • 5. We then tested three other widely used species, Epipremnum aureum (Devil’s Ivy), Schefflera ‘Amate’ (Queensland umbrella tree) and Spathiphyllum ‘ Sensation’ with similar results. Like most research projects, the findings unfolded like a detective story – following clues and piecing together the evidence. What happens with the first dose of VOC? Since we had to start somewhere, each experiment was commenced in continuous light, such as can be found in offices, hotels or shopping malls. Immediately after applying the first dose of VOC the removal rates were very slow. However, within a fairly short time (1-2 days for benzene; 4-5 days for n-hexane) they accelerated markedly. This increase in rate was in response to a ‘taste’ of the VOC. It involves the ‘switching on’ (ie induction) of a biochemical system to deal with the compound (consume / metabolise it). With further topping-up doses with either VOC this induced removal activity was maintained, or even increased further. That is, they get better with practice! Is light necessary for VOC removal? To test this question, plants were then transferred to continuous dark (lights off, black plastic over chambers). It is well known that under these conditions plant photosynthesis stops, so metabolic activity will be largely reduced to baseline ‘dark’ respiration. Stomates will also be shut, so there will be virtually no gaseous absorption into the leaves. What happens now? Does VOC removal slow down? No! The process kept on going at the same sorts of rates as in the light (Figs 1-2). In addition, when (still in the dark), new doses of VOC were injected, at even higher concentrations, (ie raised from 25 to 50 ppm for benzene and from 100 to150 ppm for n-hexane), the removal rates usually increased further as well. This indicates that with each plant species, the system remained fully operative under dark conditions, and in fact could respond to, and cope with, higher doses of each compound. In other words, we had not yet arrived at concentrations high enough to saturate the biochemical removal system (and that aspect still remains to be investigated further).
  • 6. What are the relative roles of the plant and soil micro-organisms, in the removal process? Was it the plant itself that was directly responsible for the VOC removal, even in the dark? To answer this, we removed the plants, replaced the potting mix into the pots, and put the pots back into the chambers. New standard doses of the VOC were then applied. Again, the VOC continued to disappear at rates comparable with, though generally slightly less than, those found prior to the plant's removal (Figs 1-2). After the plant’s removal, experiments were sometimes continued for a further 7 - 10 days, with top-up doses as required, and the activity was maintained in every case. The sustained activity with further doses, and in the absence of the plant, tells us two things: First, the continued activity confirms that this is a true biological response, and not merely an adsorption / absorption process. Secondly, it shows that it must be the micro-organisms of the potting mix that are the ‘rapid-removal agents’ of the pot- plant system. The plant is somehow involved, however, as discussed below. What happens when the plant is transferred to hydroponics? This was to test the plant removed from the potting mix. The roots were thoroughly washed in sterile water to remove particles of the potting mix and if possible some of the micro-organisms clinging to the surface of the roots. Nevertheless, some VOC removal sometimes continued to occur in hydroponic medium (Figs.1-2). Sometimes, though not always, the system achieved the same removal rates as in the potting mix. This suggests that the microorganisms are at least in some cases fairly firmly attached onto or inside the roots. The differences in response among the plant species in this medium suggest different relationships between the plant and the microorganisms associated with the root systems.
  • 7. What happens when unplanted potting mix is dosed with VOC? Tests with watered new potting mix, that had not been used to grow plants, showed a very slow induction when dosed with VOC, and the final induced activity was estimated to be only about half of that with plants (Fig. 3). In addition, there was some evidence of the system becoming exhausted. The results confirm what is known of potting mixes generally, namely that they contain a supply of microorganisms before plants are introduced. However, the results also suggest that the readily available nutrients for microbial growth and reproduction in the potting mix will not last very long in the absence of a growing plant. Pmx Control Expt. (plants absent throughout). 30 1 3 25 Benzene ppm 20 2 15 10 5 0 0 5 10 Day Fig.3. Benzene (Bz) levels in test chamber during control experiment with "virgin" potting mix, ie. potting mix which not previously used as substrate for plants. Each point mean ± SEM (n = 4). The bottom line – a new and improved marketing message Indoor pot plants can now be confidently promoted as helping to improve the quality of the indoor environment. The way of the future will certainly be to use them routinely for that purpose, and to ensure that buildings are designed to exploit their
  • 8. usefulness for clean air as well as for their living beauty! In summary, we can safely state that: 1. The pot-plant system really does remove VOCs from indoor air! 2. The system gets better on exposure to VOCs and maintains performance with repeated doses. 3. From 3 to 10 times the maximum permitted Australian occupational indoor air concentrations of each compound can be removed within about 24 hours, under light or dark conditions without saturating the system. 4. The pot plant system can also remove very low residual concentrations as well, - - The fact that similar responses were found with the three plant species, under all of the test conditions, indicates two things: (a), that this is a general plant- soil phenomenon, that is, it can be expected to be found with any pot-plant species; and (b) that it is the micro-organisms of the growth medium which play a primary role as the 'rapid-response agents' in VOC removal in the potted-plant system. - The plants are also involved. Comparisons of performance among the three plant species indicate that they have different substrate microbiological populations, and / or that there are different relationships between the microorganisms and the roots of the particular species. The results with new potting mix also indicate the nourishing role of the plant in promoting microbial growth. It is well established from research with crop species that different plant species develop a species-specific soil flora around their roots, producing a symbiotic microcosm of activity. It is also known that plants expend energy nourishing their substrate microorganisms, sometimes secreting from 25 to 45% of their net photosynthetic product from their roots to keep the microbes growing.
  • 9. Further work We are now working on two follow-up projects. The first is an investigation into which microorganisms, associated with these plant species and growth media, are involved in the VOC removal process. This will enable the horticultural development of plant-and-soil varieties and systems with enhanced clean-air capabilities. The second project is on the testing of these and other interior foliage plant species under flow-through conditions, to seek answers crucial questions about how much plant material, of which species will make the most impact on improving indoor air quality in the ‘real world’. For this project we will be using both test chambers of the same size as those used in the static experiments, and a scaled-up, room-sized dynamic chamber, in collaboration with associate investigator Dr. Steven Brown, at the Air Quality Laboratory of CSIRO, Melbourne. Acknowledgments We thank the Flower Council of Holland, the Horticultural Research and Development Corporation of Australia and the Nursery Industry Association of NSW via the Horticultural Stock and Nurseries Act (NSW Agriculture), for funds for this project. Thanks also to the Interior Plantscapers Association of NSW, HousePlants Australia and the Lord Howe Island Board, for plant materials and continuing interest and assistance. We also thank Ms Narelle Richardson, Laboratory Manager, and other staff and students of the Department of Environmental Sciences, UTS who have assisted in this project. References and further reading - When You Can’t Breathe, Nothing Else Matters. American Lung Association (1996), NY. - Bascom R., 1997. Plenary Paper: Health and Indoor Air Quality in Schools. Proceedings of Healthy Buildings / IAQ '97, Washington DC, 27 Sept. - 2 Oct. 1997, Vol. 1, 3-12.
  • 10. - Indoor Air Quality, Australia: State of the Environment Technical paper series (Atmosphere), Brown, SK, 1997, (a). Dept. Environment, Sport and Territories, Canberra. - Volatile organic compounds in indoor air: sources and control. Brown, SK, 1997, (b). Chemistry in Australia, Jan / Feb, 10-13. - Concentrations of volatile organic compounds in indoor air – a review. Brown, SK, Sim, MR, Abramson, MJ and Gray, CN, 1994. Indoor Air 4: 123- 134.1994; - Home and workplace: complaints and symptoms in office workers and correlation with indoor air pollution. Carrer, P, Alcini, D, Cavallo, D, Visigalli, F, Bollini, D and Maroni, M, 1999. In, Proceedings of 8th international Conference on Indoor air Quality and Climate, Edinburgh, Scotland, 129-134. - Pilot Study to Assess the Impact of Green Plants on NO2 levels in Homes. Coward M, Ross D, Coward S, Cayless S and Raw G, 1996. Building Research Establishment Note N154/96. Watford, UK. - Detoxification of formaldehyde by the Spider Plant (Chlorophytum comosum L.) and by soybean (Glycine max L.) cell suspension cultures. Giese, M., Bauer- Dorancth, U, Langerbartels, C, Sandermann Jr, H, 1994. Plant Physiology 104: 1301 - 1309) - Particulate matter accumulation on horizontal surfaces in interiors: influence of foliage plants. Lohr VI and Pearson-Mims CH, 1996. Atmospheric Environment 30: 14, 2565-2568. - Exposure Standards for Atmospheric Contaminants in the Occupational Environment. National Occupational Health and Safety Commission (Aust), 1991. AGPS, Canberra, Australia. - Draft National Protection Measure and Impact Statement for Ambient Air Quality, NEPC (National Environment Protection Council) (1997). NEPC Service Corp. Adelaide p.101 - Metropolitan Air Quality Study-Outcomes and Implications for Managing Air Quality. NSW EPA (1996) EPA 96/20; Chatswood NSW. - Proceedings of Health and Urban Air Quality in NSW Conference, Sydney June 3-4 Vol I, II. NSW Health Dept (1996) NSW Health Dept. Gladesville NSW.
  • 11. - Air Pollution and Plant Metabolism. Schulte-Hostede S, Darrall NM, Blank LW and Wellburn AR (Eds), 1987 Elsevier, NY. - Rhizospheric hydrocarbon-utlizing microorganisms as potential contributor to phytoremediation for the oily Kuwait desert. Radwan, SS, Al-Awadhi, H., Sorkhoh, NA and El-Nemr, IM, 1998. Microb Res 153: 3, 247 – 251. - Higher plant metabolism of xenobiotics; the ‘green liver’ concept. Sandermann H., Jr, 1994. Pharmacogenetics 4: 225-241. - Adsorption of naphthalene onto plant roots. Schwab, AP, Al-Assi, AA and Banks, MK,1998. J Environ Qual 27: 1, 220 - 224). - Interior Landscape Plants for Indoor Air Pollution Abatement, Final Report, Sept., Wolverton BC, Johnson A and Bounds K, 1989. NASA Stennis Space Centre MS. - Removal of Formaldehyde from Sealed Experimental Chambers, by Azalea, Poisettia and Dieffenbachia. Wolverton Environmental Services INc., 1991. Res. Report No. WES/100/01-91/005. - Eco-Friendly House Plants. Wolverton BC 1996. Weidenfeld and Nicolson, London. - Living plants to improve indoor air quality. Wood RA, Orwell RL and Burchett MD,1998. In, MD Burchett, J. Tarran and R Wood (eds). Towards a New Millennium of People-Plant Relationships, Contributions from the International People Plant Symposium, Sydney, Australia July. 115-122 - Absorption of organic compounds in indoor air by commonly used indoor plants. Wood, R. A., Orwell, R., and Burchett, M. D., Tarran, J. and Brown, SK, 2000. Proceedings of Healthy Buildings 2000, Espoo, Finland, Aug 6- 10, Vol 2, 125-130. - Potted plant-growth media: interactions and capacities in removal of volatiles from indoor air. Wood, R. A., Orwell, R., Tarran, J., Torpy F., and Burchett, M. D., 2002. Journal of Environmental Horticulture and Biotechnology. 77: (1) 120-129.