A Radioisotope Assay for the Quantification of Hydrocarbon Biodegradation Potential in Environmental Samples D. M. CAPARELLO AND P. A. LAROCK Department of Oceanography, Florida State University, Tallahassee, bTorida 32306

Abstract

An enrichment culture method is described for quantifying the activity of hydrocarbon oxidizing bacteria in water and sediments. Application of the procedure indicated that the hydrocarbon oxidizing potential of environmental samples reflects the hydrocarbon burden of the area, the ability of the microflora to utilize hydrocarbons, and that lakes with large aquatic plant communities contain populations of hydrocarbon bacteria comparable to those found in oil-polluted harbors. Introduction

During the past 50 years at least five million tons of petroleum have been spilled into the sea (Pilpel, 1968). Currently, maritime spillage is estimated to be five to ten million tons per year while the volume of hydrocarbons derived from terrestrial sources such as road runoffs, and industrial effluent is approaching similar magnitudes (Blumer, 1968). This input, however, has not resulted in any great accumulation of oil. The disappearance is the result primarily of natural degradation measures initiated first by sunlight and followed by microbial biodegradation [11 ]. Microbial hydrocarbon oxidizers are widely distributed on land and coastal waters, particularly in areas subject to frequent oil pollution (ZoBell [20]). Measurements of microbial hydrocarbon oxidation have been made using a variety of procedures including bacterial enumeration techniques (Davis [8]; Gunkel [12]), respirometric methods (Davis [8]; Jones [14, 15]; Davies and Hughes [7] ), labeled hydrocarbons (Davis and Raymond [9]), infrared spectrophotometry (Davis [8]), and oxygen electrodes (Buswell and Jurtshuk [5]). Each of these methods has its limitations. Infrared methods seem to be consistent for oils high in aliphatics but less suitable for lower members of the aromatic series (Floodgate [10]). Manometric techniques are subject to vapor pres28 MICROBIAL ECOLOGY, Vol. 2, 28-42 (1975) 9 1975 by Springer-Verlag New York Inc.

Radioisotope Assay for Quantification of Hydrocarbon Biodegeneration Potential

29

sure limitations when used with some hydrocarbons (Floodgate [10]). Davis [8] found manometric procedures to be complicated systems often requiring 5 to 30 days to obtain measurements for ethane oxidizing bacteria. Bacterial enumeration procedures have been described by several investigators. Gunkel [12] used a high speed homogenizer with an emulsifier to prepare serial dilutions for the Most Probable Number estimates. Davis [8] cites several advantages for the plate count technique, but Jones and Edington [16] found plating to be unwieldy owing to the precautions necessary to insure that the agar be free of organic impurities. Plate counts may even result in the emergence of cultures that in the natural habitat are of minor significance in oxidizing hydrocarbons. Jones [15] used a buried slide technique to enumerate hydrocarbon oxidizers in soils. He concluded, however, that population studies in microbial oil degradation were less useful than the measurement of oxidizing activity since bacterial numbers yield no information on the rate of microbial oil degradation. Gunkel [12] had arrived at the same conclusion. The purpose of this paper is to describe a simple enrichment assay procedure that permits a rapid quantification of bacterial hydrocarbon oxidizing activity in natural environments. Material and Methods

Cultural Procedures Marine hydrocarbon oxidizing bacteria were grown on enriched seawater (ENSW) composed of (NH4) 2SO4, l0 ppt; K2HPO4, 50 ppm; and yeast extract, 0.1% in artificial seawater ("Instant Ocean," Aquarium Systems Inc., Wickliffe, Ohio). Freshwater bacteria were grown on Bushnell and Haas mineral salts medium (BH), supplemented with 0.1% yeast extract (Bushnell and Haas [4]). Estuarine bacteria were grown on BH medium to which 1.0% NaC1and 0.05% yeast extract were added. When a solid medium was desired for plate counting, 1.5% agar was added to the appropriate basal salts medium. The hydrocarbon source was Fisher heavy paraffin oil and Fisher kerosene (PK) mixed 1:1 v/v and was added to the lids of inverted Petri dishes. Cultures for laboratory experiments were isolated from marine and freshwater environments or~ the appropriate medium except the yeast extract concentration was lowered to 0.01%. After isolation, cultures were maintained on slants of the appropriate agar medium with 1 ml of sterile PK pipetted on the agar surface. The two hydrocarbon sources uscd were 14Ci-hexadecane (14C-16) and a synthetic mixture of commercially available n-alkanes varying in chain length from C-t0 to C-25 (HC MIX). HC MIX was prepared so that the lower molecular weight alkanes (C-10 to C-17) were present in twice the concentration of C-18 to C-25 to maintain the complete mixture as a liquid at room temperature.

Sample Collection Water and slick samples were collected by skimming the surface with a sterile "Whirl-pak." Sediment samples were collected by inserting sterile 8 mm diam. glass core tubes into the sediments and then plugging the ends with sterile corks. All samples were refrigerated until assayed, which was usually within 12 hr after collection.

30

D . M . Caparello and P. A. LaRock

Determination of biomass by adenosine triphosphate (ATP) was made according to the method of Quammen et aL[ l 9].

Measurement o f Microbial Hydrocarbon Oxidation 1. Radioisotope Assay. Bacterial hydrocarbon oxidizing activity was measured by collecting tile 14CO 2 evolved from the oxidation of 14C1-16. The procedure used was patterned after the technique of Harrison et al. [13] with minor modifications to permit the use of hydrocarbons. In place of serum bottles, 50 ml Erlenmeyer flasks were used, each having 4 glass vanes indented around the base to assure mixing and dispersal of the hydrocarbon in the basal medium. The Erlenmeyer flasks also minimized splashing of the medium onto the filter paper CO 2 trap at the high shaking rates used. In application, a series of 50 ml Erlenmeyer flasks containing 10 ml of either BH or ENSW media were sealed with aluminum foil and autoclaved for 20 rain at 15 psi. Next, 1 ml of the sample to be assayed, either a suspension of a pure culture or environmental sample, was added to each test flask. Sediment inocula were prepared by first withdrawing the overlying water in the corer to within l cm of the sediment. The sediment was extruded and discarded until only the top 2 cm of sediment remained in the corer. This surface sediment was emptied into a reaction flask with a separate core of each sample used to inoculate the desired number of flasks. Twenty-five microliters of 14C-16 with a specific activity of 2 )< 106 dpm/ml was then added to the water surface of each flask using a 50 ~1 syringe (Hamilton Corp.). Repetitive testing indicated that this method of adding hydrocarbons was highly reproducible for a given operator. The flasks were sealed with a rubber stopper (Priezer Scientific, Philadelphia, Pa.) fitted with a center well and Filter paper assembly (Harrison et al. [13]) and incubated at 35~ on a gyrotory shaker at 240 rpm. Uninoculated flasks served as controls. After the desired incubation time, duplicate growth flasks and controls were sacririced by injecting 0.2 ml of &phenethyla_mine on the filter paper, followed by 2.0 ml of 1 N H2SO 4 into the medium to stop the reaction and release the CO 2. After acidification, the flasks were shaken for an additional hour to permit absorption of the I4CO 2. The filter paper was removed, placed in 15 ml of Aquasot (New England Nuclear, Boston, Mass.), and counted on a Nuclear Chicago Model 4534 liquid scintillation counter. Quench was corrected for by the channels ratio method. The activity of duplicate flasks was averaged and the 14CO 2 evolved expressed as a percentage of the activity initially added as 14C-16 according to the following equation: dpm (experimental filter) - dpm (control filter) • 100 Percent 14CO2 evolved -

dpm (14C-16 added)

The 14CO 2 evolved was expressed as a percentage of the activity added to compensate for variations in specific activity of different batcfies of the hexadecane. 2. Gravimetric Assay for the Determination o f n-Alkane Oxidation. In batch culture experiments using HC MIX, hydrocarbon loss was determined gravimetrically. Duplicate 125 ml Erlenmeyer flasks, each containing 20 ml of ENSW for marine bacteria, or 20 ml of BH for freshwater organisms, were inoculated with 1 ml of a suspension of the desired culttue to give a final density of 5 • 106 cells]ml. Next, 50 pl of HC MIX were added with a syringe, the flasks plugged with cotton and sealed with aluminum foil, The flasks were incubated at 35~ for 24 hr on a gyrotory shaker operating at 160 rpm. After incubation, 1 pl

Radioisotope Assay for Quantificafioz~ of Hydrocarbon Biodegeneration Potential

31

of 14C_16 in a hexane solvent was added to the reaction flasks followed by 20 ml of hexane for the extraction of the residual hydrocarbons. The radioisotope was used to determine the efficiency of the extraction process and had an activity of approximately 10,000 dpm/td, The/]asks were shaken for t hr and the phases separated. The hexane containing the remaining HC MIX was concentrated under a stream of nitrogen to 2.5 ml in calibrated glassstoppered centrifuge tubes. Next, 0.5 ml of this solution was withdrawn and counted using 15 ml of Aquasol and the efficiency of the extraction determined. The remaining solution was transferred to a tared aluminmn weighing dish, the hexane evaporated under nitrogen, and the dishes reweighed on a Mettler HI6 balance. The percentage of the hydrocarbons oxidized was calculated from the following equation: Percent hydrocarbon oxidized

0 . 8 N W - WJ x 10 2 0.8 NW

where N = extraction efficiency W = weight of 50 #1 of HC MIX 14[/ = weight of residual HC MIX.

Generation o f Growth Curves The effect of inoculmn density on culture outgrowth under conditions used in the radioassay was studied for several pure cultures and enviromnental samples. Environmental samples were used directly to inoculate the growth flasks. Pure cultures were pregrown on the appropriate agar and incubated for 24 hours at 35~ The cells were harvested with BH or ENSW medium and the suspension brought to an optical density of 0.3 at 610 rim. This yielded a suspension containing between 2 X 108 to 2 X 109 cells/ml depending on the organisms used. The desired inoculum density was obtained by serial dilutions to cover a range of 2.2 x 103 to 2.2 • 106 cells/flask, using ml inoculum size of 1 ml. Preparation of the growth flasks and their analysis was carried out as described in the radioisotope assay except that duplicate flasks of each sample were sacrificed at the first indication of turbidity and at 2 - 4 hr intervals thereafter. The experiment was terminated after 30 hr.

Results In the radioassay, we a s s u m e d n - h e x a d e c a n e c o u l d replace a m i x t u r e o f n-alkanes as a h y d r o c a r b o n s u b s t r a t e w i t h o u t a f f e c t i n g the relative q u a n t i t y o f h y d r o c a r b o n o x i d i z e d . We f u r t h e r a s s u m e d t h a t t h e ~4CO2 evolved w o u l d serve as an a c c u r a t e m e a s u r e o f t h e h y d r o c a r b o n utilized. T o test this rationale, a series o f test c u l t u r e s h a v i n g v a r y i n g ability t o utilize h y d r o c a r b o n s ( T a b l e 1) were g r o w n u s i n g 14C-16 u n d e r t h e c o n d i t i o n s o f the radioassay a n d w i t h a m i x t u r e o f n - a l k a n e s u n d e r the c o n d i t i o n s o f t h e g r a v i m e t r i c assay. All flasks were i n c u b a t e d 2 4 hr. In Fig. 1, t h e results o f t h e t w o assay m e t h o d s have b e e n p l o t t e d against o n e a n o t h e r . B o t h m e t h o d s r a n k e d t h e test c u l t u r e s in t h e s~une o r d e r a c c o r d i n g to their ability to use t h e respective h y d r o c a r b o n s u b s t r a t e . T h e l i n e a r i t y o f t h e p o i n t s i n d i c a t e s t h a t , n u m e r i c a l l y , the m a g n i t u d e o f the r e s p o n s e e a c h m e t h o d

32

D. M. Caparello and P. A. LaRock Table 1 Test Cultures and Location o f Isolation Culture

Area of isolation

FHR-2

Surface water from the Fenholloway River, Perry, Florida

LM-1

Surface water from Lake Munson, Tallahassee, Florida

LM-2

Surface water from Lake Munson

HR-2

Surface water from Hillsborough River, Tampa, Florida

C-5

Beach sand from Coal Oil Point, California

L-2

Surface oil slick in Barataria Bay, Louisiana

C-22

Water from Boston Harbor, Boston, Massachusetts

12

HR-2 10

>.

8-

~LM-2

2"

6 1'0 1'4 1'8 22 26 3"0 Percent HC MIX degraded - gravimetrie determination

3'4

Fig. 1. Comparison of the radioisotope assay and gravimetric technique as measures of hydrocarbon oxidation by pure cultures, lnoculum size for each culture was 10 8 cells.

Radioisotope Assay for Quantification of Hydrocarbon Biodegeneration Potential

33

measures is directly proportional. Hexadecane may therefore substitute for a mixture of n-alkanes, and the 14C02 evolved is a measure of the ability of the test culture to oxidize n-alkanes. The growth characteristics and rates of 1 4 C O 2 evolution of active and nonactive hydrocarbon oxidizers were examined using the radioassay (Fig. 2). The 14CO2 evolved for each culture indicated that the active oxidizer, HR-2, had a much higher stationary phase 14CO2 evolution than either C-22 or C-5. The length of the lag and slope of the exponential phases of each culture varied. The more active oxidizer had the greatest log phase slope and the shortest lag time. The weakest oxidizer, C-5, had the smallest log phase slope and the longest lag 9 time. The inoculum density for C-5 was 3.3 X 108 cells/flask, for C-22 it was 4.1 • 108 cells/flask, and for HR-2 it was 2.2 X 104 cells/flask. A family of growth curves was generated using the radioassay for the active oxidizer HR-2 over an inoculum range of 2.2 X 103 to 2.2 • 106 cells/flask (Fig. 3). All inoculated flasks eventually reached the same stationary phase cell density and 14CO 2 evolution. The length of the lag time for each curve was inversely proportional to the logarithm of the inoculum density (Fig. 4). The displacement of the growth curve, or more precisely the length of the lag period, is therefore a measure of the size of the bacterial population in the original sample. Varying the inoculum density for a given culture did not affect the slope of the 12 A

10

O~ 6

HR-2

~,

C-22

n

2

0

;I

I

I

I

I

I

I

I

|

I

10

12

14

16

18

20

22

24

26

28

30

Time, hr

Fig. 2. Growth characteristics and rates of 1 4 C O 2 evolution for three pure cultures of varying hydrocarbon oxidizing activity. The cultures were HR-2, C-22, and C-5 with inoculum densities of 2.2 X 10 4, 4.1 • 108, and 3.3 X 108 cells/ flask, respectively.

34

D . M . Caparello and P. A. LaRock

exponential phase or the quantity of 14CO2 evolved when the culture reached the stationary phase. The growth characteristics of environmental samples were investigated by generating a set of growth curves similar to those of the pure culture experiment. Water samples (Table 2, sample 4) were collected from the Sparkman ship canal in Tampa Bay, Florida and used as an inoculum full strength, and with 5-, 10-, and 102-fold dilutions. The resultant growth curves (Fig. 5) had the same basic features of the pure culture experiment. The length of the lag phase was inversely proportional to the logarithm of the inoculum density, each curve had a similar slope for the exponential phase, and the same quantity of 14CO2 was evolved when the cultures reached the stationary phase. The hydrocarbon oxidizing activity of the microflora in a number of environmental samples was measured using the radioassay. In these experiments, 1 ml of aqueous sample or a single core (1 cc total volume) was added to a series of reaction flasks and incubated for 24 hours. The 14CO2 evolved in this incubation period is presented in Table 2 and suggests the oxidizing potential of an environmental sample may reflect the degree of hydrocarbon addition to which the area is subjected. Sample 1 had the greatest ~4CO 2 evolved by the water samples but the activity of the freshwater samples surpassed most of the estuarine and marine samples. Comparison of the 14CO2 evolved and ATP biomass of samples 1, 4, 5, 6, and 7 indicated that samples from areas of relatively little hydrocarbon burden (samples 6 and 7) had less 14CO 2 evolved than polluted areas did (samples 1, 4, and 5). Estimates of biomass using ATP will indicate only the total microbial population irrespective of what elements compose the microflora. A

~

12

,8

E

F

G

6, .4 . ,2,1..5 ,,8,,6,4, , 2!.~.86 4. ,2!~

106

105

104

103

10 2

E 4 2 L

I

I

I

L

1

I

I

1

I

t

I

I

0

2

4

6

8

10

12

14

16

18

20

22

24

-~

26

[

28

30

Time, hr

Fig. 3. T h e effect of v a r y i n g t h e i n o c u l u m d e n s i t y o n the p e r c e n t J 4CO2 evolved

by culture HR-2. The inoculum density for the family of curves is: A, 2.2 X 106; B, 1.7X 106; C, 1.1 X 106;D, 5.5 X 10s; E, 2.2X IOS;F, 2.2X 104;G, 2.2X 103 cells/flask. The log scale insert is used to interpolate between curves.

Radioisotope Assay for Quantification of Hydrocarbon Biodegeneration Potential

35

Samples 1 and 6 had nearly equivalent biomass but the 1 4 C 0 2 evolved by sample 6 was one-tenth that of sample 1. Analysis of sand (samples 8 to 12) showed the same trend as was found with the corresponding water samples. However, a greater amount of 14CO2 was evolved than was found with the water samples. This is seen by comparing samples 1, 4, 5, and 6 to samples 8, 9, 10, and 12, respectively. The most active samples were cresote scrapings collected from dock pilings (samples 13 and 14). 7

-8 E o

_J

3

I

0

1

5

1

1

1

10 Time, hr, for 5%

15

20

25

30

14C02 evolved

Fig. 4. Duration of the lag phase for culture HR-2 as a function of the log of inoculum density.

0%

4

Sample

16.0

17.0

Cove in Sparkman channel; near shore surface water; little or no slicks observed; receives sewage effluent

Cove adjacent to location 4; near shore surface water; receives sewage effluent; no oil slicks observed

2.9 X 10 6

2.0

2.5

4.4

11.7

(percent)

i 4CO 2 Evolved

Lake Jackson, Tallahassee, Fla.; shore surface water; no slicks observed; large plant population 3 . 6 X 10 6

count (cells m l - 1)

9.9

5.0

ATP Concentration (/ag l i t e r - 1)

Lake Munson, Tallahassee, Fla. ; near shore surface water, surface slicks present; receives city treated sewage; large algal and plant population

Sparkman ship channel, Tampa Bay, Fla.; near shore surface water; prominent surface oil slicks; active shipping activity in channel

Location and description

Plate

Table 2 Location and Description o/Environmental Samples Tested with the Radioassay

3.2 X 10 3

3.6 X 10 a

5.5 X 10 3

1.5 X 10 4

> 10 s

Radioassay estimated population (cells m l - 1)a

< 10 3

0.1

0.2

Outside m o ut h of Tampa Bay, Fla.; surface water; no oil slicks; clear open Gulf water

4.5 X 10 3 10 s l0 s

6.1

3.5 16.6 11.2

2.4 X 10 6

Same site as sample 10, 3 days later, no surface oil slicks observed at this sampling

Near shore sand at location of sample 6

Scrapings from dock pilings in Tampa Bay

Creosote ooze from dock pilings in Tampa Bay

11

12

13

14

aEquivalent cell density of inoculum.

8.2 X 10 3

9.0

3.2 X 10 6

Near shore sand at location of sample 5

10 F

12.2

8.3 X 10 6

Near shore sand at location of sample 4

9

1.5 X 10 4

lO s

12.8

2.7 X 10 6

Near shore sand at location of sample 1

lO s

2.0 X 10 3

1.1

3.2

Hillsborough River, Tampa, Fla.; midriver surface water; no slicks or heavy plant growth observed; light boat traffic

8

6

38

D.M. Caparello and P. A. LaRock

02

8

1

o.

I 0

I 2

I 4

I 6

I 8

I I 10 12 Time, hr

I 14

I 16

I 18

I 20

i 22

24

Fig. 5. The effect of varying the inoculum density on the percent 14CO 2 evolved by an environmental surface water sample from Sparkman Channel, Tampa Bay, Florida. The inoculum density for the family of curves is: A, 3.6 X 106; B, 2X 105;C, 3.6 X 105;D, 3.6 • 104 cells/ml. In comparing the radioassay estimations (for a 24 hr incubation period) to ATP biomass and plate counts (Table 2), it is seen that the biomass for sample 1 was less than for samples 4 and 5, but the 14CO z evolved was five times greater. Similarly, plate counts of samples 8, 10, and l 1 were equivalent to samples 4 and 5 but their 1 4 C O 2 evolved was three to five times greater. This suggests that the hydrocarbon oxidizing potential of a sample is a function of the oxidizing activity of the microflora as well as its cell density. Discussion

In the enrichment culture technique described, the important parameters of bacterial development are (1) the quantity of 14CO 2 evolved is a measure of the amount of hydrocarbon oxidized (Fig. 1); (2) the quantity of 14CO2 evolved is a measure of the culture's ability to utilize hydrocarbons (Fig. 2); (3) the length of the lag phase of growth is a function of the inoculum density. The more cells added to the growth flasks, the shorter the lag period (Fig. 3); and (4) the quantity of CO2 evolved in the stationary phase for a given culture is independent of the inoculum density, but for smaller inocula a longer incubation period is required to attain this final 14CO 2 concentration (Figs. 3 and 4). These features permit the radioassay to be used to quantify hydrocarbon oxidizing activity in two ways. The first method merely measures the 14CO2 released after a fixed incubation period and thus indicates the relative ability of the sample to degrade hydrocarbons. For example, if the cultures shown in Fig. 2

Radioisotope Assay for Quantification of Hydrocarbon Biodegeneration Potential

39

were assayed at 24 hr, the ability of each to oxidize hydrocarbons would be proportional to the amount of 14CO2 evolved during the fixed incubation period. On this basis, culture HR-2 would be found to be the strongest oxidizer and the C-5 the weakest. When used with environmental samples, the amount of 14CO 2 released in a fixed incubation period is thus a relative measure of the ability of the specified sample to assimilate hydrocarbon materials. The second method for using the radioassay introduces time as an additional variable, thereby extending the range of the tectmique. In general, the duration of the lag phase of growth in a batch culture is inversely proportional to the logarithm of tile cell density in the inoculum (Lamanna and Mallette [17]). Using a hydrocarbon oxidizing bacterium (Culture HR-2, Table 1), a series of growth curves were generated for inocula of different sizes (Fig. 3) and" the duration of the lag was found to be proportional to the logarithm of the inoculum density under the conditions of the radioassay (Fig. 4). The duration of the lag phase may thus be used to arrive at a numerical estimate of the cell density in the inoculating material. Under this condition the growth curves of Fig. 3 are used to translate differences in lag into population estimates. Using the incubation time and 14CO2 evolved by an environmental sample or test culture, a point is located within the family of standard curves (Fig. 3), and a numerical estimate of the bacterial population is read off the curves. The cell density so obtained is, in reality, the inoculum density of the standardizing culture that will produce an equivalent amount of 14CO 2 in the same incubation period, and not the actual population density contained in the sample. This technique permits comparison of the hydrocarbon oxidizing activity of different environments made up of different populations. The laboratory culture used to generate the standard curves serves only to provide a base for comparing environmental samples. The actual activity of the standardizing culture is not important. In using Fig. 3 to estimate the number of hydrocarbon bacteria in a sample, one must consider that the radioassay indicates only that the quantity of 14CO2 evolved by a sample can be produced in the same period of time by a laboratory culture of known inoculum density. Thus, a large population of less active oxidizers and another smaller, but more active population could produce similar amounts of 14CO 2 and therefore be interpreted as equal populations. Numerically, the populations are not equivalent, but their ability to assimilate hydrocarbons is. Application of the radioassay to environmental samples collected in and around Tampa Bay and in two North Florida lakes indicated that hydrocarbon oxidizing bacteria are ubiquitous. They were found in water and sediment in both unpolluted and oil polluted areas, as had previously been reported (ZoBell [20, 21]). The abundance of oil degrading bacteria, however, was greatest in areas receiving waste hydrocarbon materials. The water sample taken from a ship canal in Tampa Bay, where there were visible oil slicks, (Table 2, sample 1), had

40

D . M . Caparello and P. A. LaRock

greater hydrocarbon utilizing populations than did the Hillsborough River which feeds into the bay (sample 6) or the Gulf of Mexico at the mouth of the bay (sample 7). The total microbial biomass, as estimated by ATP, for samples 1,4, 5, and 6 varied by a factor of 5. The hydrocarbon utilizing population, however, varied by a factor of at least 50 (Table 2). The enhanced hydrocarbon oxidation observed for sample 1 indicates that for a given microbial biomass, exposure of the sample to oil will either increase the hydrocarbon utilizing component or replace the existing bacterial component by another population that is more adapted to oxidize oil. The low hydrocarbon oxidizing activity and high ATP content of samples 4 and 5, relative to sample 1, may be the result of the addition of the effluent of a sewage treatment plant. Under similar conditions in Raritan Bay, N.J., Atlas and Bartha [2] reported a substantial increase in the total number of microorganisms at a sewage outfall, but no change was noted in the numbers of oil oxidizing bacteria. Atlas and Bartha [1 ] further indicated that low phosphate and nitrate concentrations are limiting factors in the microbial degradation of hydrocarbons, particularly in seawater. They found that no observable microbial oil degradation occurred within 18 days in offshore water with 0.98 rag/liter nitrogen and .07 mg]titer phosphorous. The nitrate-nitrogen and phosphate-phosphorous concentrations in sample 7 were 0.158 mg/liter and 0.067 mg/liter, respectively. The low oxidizing activity at this location may be the result of either low nutrient concentrations or a microbial population that was relatively inactive for hydrocarbon oxidation. In Tampa Bay proper neither nitrates or phosphates are limiting as a result of the discharge of sewage and the wastes from phosphate mining. The analysis of sediment or sand samples (Table 2, samples 8 - 12) indicates that areas with higher hydrocarbon burdens have greater hydrocarbon oxidizing activity and that sediments have larger hydrocarbon utilizing populations than the overlying water. Similar results have been reported by Colwell et al. [6] in Chesapeake Bay where sediments from oil polluted areas contained as much as 100 times more oil utilizing bacteria than did the overlying water. Of great interest was the finding that freshwater lakes contain hydrocarbon utilizing populations of comparable magnitude to those found in oil polluted estuarine environments. Lake Munson receives the effluent from a sewage treatment plant and the nutrients added to the lake have resulted in the development of water plants and frequent heavy algal blooms. At times visible oil slicks are present which could originate either from grease and oils in the sewage or from plant hydrocarbons. Lake Jackson is located in a relatively undeveloped area and as such receives runoff from predominantly wooded land. At present we can only speculate that the hydrocarbon oxidizing activity found in these lakes may be in response to material contributed primarily as plant hydrocarbons, although a more exhaustive study is necessary to resolve this question.

Radioisotope Assay for Quantification of Hydrocarbon Biodegeneration Potential

41

Acknowledgments Dominic M. Caparcllo was supported by NSF Grant GZ-2337 to Florida State University. Samples were collected in Tampa Bay aboard the R. V. Tursiops through funds provided by the NSF under Contract GC-28174.

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2.

Atlas, R. M., and Bartha, R. 1973. Abundance, distribution and oil biodegradation potential of microorganisms in Raritan Bay. Environ. Pollut. 4:291 - 300.

3.

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4.

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5.

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6.

Colwell, R. R., Walker, J. D., and Nelson, J. D. 1973. Microbial ecology and the problem of petroleum degradation in Chesapeake Bay. ln: The Microbial Degradation o f Oil Pollutants. D. G. Ahearn and S. P. Meyers, editors. Center for Wetland Resources, Louisiana State Univ. Publ. No. LSU-SG-73-01. pp. 185 -197.

7.

Davies, J. A., and Hughes, D. E. 1968. The biochemistry and microbiology of crude oil degradation, ln: Field Studies Council Symposium. The Biological Effects o f Oil Pollution on Littoral Communities. Carthy and Arthur, editors. Field Studies Council, London, pp. 139 - 144.

8.

Davis, J. B. 1967. Petroleum Microbiology. Elsevier, New York, 604 pp.

9.

Davis, J. B., and Raymond, R. L. 1961. Oxidation of alkyl substituted cyclic hydrocarbons by a Noeardia during growth on n-alkanes. Appl. Microbiol. 9: 383 - 388.

10.

Floodgate, G. D. 1972. Biodcgradation of hydrocarbons in the sea. In: Water Pollution Microbiology. R. Mitchell, editor. Wiley-lnterscience, New York. pp. 153 - 171.

ll.

Friede, J., Quire, P., Gholson, R., Gaudy, E., and Gaudy, A. F. 1972. Assessment of biodegradation potential for controlling oil spills on the high seas. Project 4110.1/3.1, Dept. of Transportation. 130 pp.

12.

Gunkel, W. 1968. Bacteriological investigations of oil polluted sediments from the Cornish coast following the Torrey Canyon disaster, ln: Field Studies Council Symposium. The Biological E lfeets o]" Oil Pollution on Littoral Communities. Carthy and Arthur, editors. Field Studies Council, London, pp. 115 - 158.

13.

ttarrison, M. J., Wright, R. T., and Morita, R. Y. 1971. Method for measuring mineralization in lake sediments. Appl. Microbiol. 21:698 - 702.

14.

Jones, J. G. 1968. Methods of studying the effect and metabolism of hydrocarbons in natural environments, hT: Field Studies Council Symposium. The Biological

42

D.M.

CapareUo and P. A. LaRock

Effects o f Oil Pollution on Littoral Communities. Carthy and Arthur, editors. Field Studies Council, London, pp. 145 - 150. 15.

Jones, J. G. 1969. The determination of microbial h y d r o c a r b o n metabolism in natural environments. Arch. Microbiol. 6 7 : 3 9 7 - 407.

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A radioisotope assay for the quantification of hydrocarbon biodegradation potential in environmental samples.

An enrichment culture method is described for quantifying the activity of hydrocarbon oxidizing bacteria in water and sediments. Application of the pr...
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